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Document 01979D0542-20040501

    Consolidated text: Council Decision of 21 December 1976 drawing up a list of third countries or parts of third countries, and laying down animal and public health and veterinary certification conditions, for importation into the Community of certain live animals and their fresh meat (79/542/EEC)

    ELI: http://data.europa.eu/eli/dec/1979/542/2004-05-01

    1979D0542 — EN — 01.05.2004 — 012.002


    This document is meant purely as a documentation tool and the institutions do not assume any liability for its contents

    ►B

    ▼M54  COUNCIL DECISION

    of 21 December 1976

    drawing up a list of third countries or parts of third countries, and laying down animal and public health and veterinary certification conditions, for importation into the Community of certain live animals and their fresh meat

    (79/542/EEC)

    (OJ L 146, 14.6.1979, p.15)

    Amended by:

     

     

    Official Journal

      No

    page

    date

     M1

    COMMISSION DECISION of 4 May 1979

      L 147

    49

    15.6.1979

     M2

    COMMISSION DECISION of 2 March 1984

      L 70

    18

    13.3.1984

     M3

    COMMISSION DECISION of 2 October 1985

      L 278

    35

    18.10.1985

     M4

    COMMISSION DECISION of 17 October 1985

      L 293

    17

    5.11.1985

     M5

    COUNCIL DECISION of 19 December 1985

      L 372

    28

    31.12.1985

     M6

    COMMISSION DECISION of 29 July 1986

      L 243

    34

    28.8.1986

     M7

    COMMISSION DECISION of 14 December 1988

      L 7

    27

    10.1.1989

     M8

    COMMISSION DECISION of 16 July 1990

      L 193

    36

    25.7.1990

     M9

    COMMISSION DECISION of 27 September 1990

      L 267

    46

    29.9.1990

     M10

    COMMISSION DECISION of 14 June 1991

      L 195

    43

    18.7.1991

     M11

    COMMISSION DECISION of 17 December 1991

      L 8

    12

    14.1.1992

     M12

    COMMISSION DECISION of 5 March 1992

      L 71

    27

    18.3.1992

     M14

    COMMISSION DECISION of 9 March 1992

      L 71

    30

    18.3.1992

     M15

    COMMISSION DECISION of 14 April 1992

      L 124

    42

    9.5.1992

     M16

    COMMISSION DECISION of 2 July 1992

      L 197

    70

    16.7.1992

     M17

    COMMISSION DECISION of 22 December 1992

      L 40

    17

    17.2.1993

     M18

    COMMISSION DECISION of 19 January 1993

      L 40

    23

    17.2.1993

     M19

    COMMISSION DECISION of 6 April 1993

      L 108

    129

    1.5.1993

     M20

    COMMISSION DECISION of 17 May 1993

      L 138

    11

    9.6.1993

     M21

    COMMISSION DECISION of 27 July 1993

      L 201

    28

    11.8.1993

     M22

    COMMISSION DECISION of 26 January 1994

      L 27

    53

    1.2.1994

     M23

    COMMISSION DECISION of 18 May 1994

      L 137

    72

    1.6.1994

     M24

    COMMISSION DECISION of 29 June 1994

      L 187

    11

    22.7.1994

     M25

    COMMISSION DECISION of 27 July 1994

      L 214

    17

    19.8.1994

     M26

    COMMISSION DECISION of 18 July 1995

      L 181

    42

    1.8.1995

     M27

    COMMISSION DECISION of 25 July 1995

      L 190

    9

    11.8.1995

     M28

    COMMISSION DECISION of 25 July 1995

      L 190

    11

    11.8.1995

     M29

    COMMISSION DECISION of 26 January 1996

      L 30

    52

    8.2.1996

     M30

    COMMISSION DECISION of 26 February 1996

      L 107

    1

    30.4.1996

     M31

    COMMISSION DECISION of 11 October 1996

      L 267

    29

    19.10.1996

     M32

    COMMISSION DECISION of 17 October 1996

      L 279

    33

    31.10.1996

     M33

    COMMISSION DECISION of 12 December 1996

      L 3

    9

    7.1.1997

     M34

    COMMISSION DECISION of 14 February 1997

      L 62

    39

    4.3.1997

     M35

    COMMISSION DECISION of 14 October 1997

      L 295

    37

    29.10.1997

     M36

    COMMISSION DECISION of 6 February 1998

      L 46

    8

    17.2.1998

     M37

    COMMISSION DECISION of 6 October 1998

      L 286

    53

    23.10.1998

     M38

    COMMISSION DECISION of 27 October 1998

      L 296

    16

    5.11.1998

     M39

    COMMISSION DECISION of 5 March 1999

      L 83

    77

    27.3.1999

     M40

    COMMISSION DECISION of 17 March 1999

      L 87

    13

    31.3.1999

     M41

    COMMISSION DECISION of 30 April 1999

      L 117

    52

    5.5.1999

     M43

    COMMISSION DECISION of 26 July 1999

      L 211

    53

    11.8.1999

     M44

    COMMISSION DECISION of 5 November 1999

      L 300

    30

    23.11.1999

     M45

    COMMISSION DECISION of 17 December 1999

      L 1

    17

    4.1.2000

     M47

    COMMISSION DECISION of 14 February 2000

      L 51

    41

    24.2.2000

     M48

    COMMISSION DECISION of 24 February 2000

      L 64

    22

    11.3.2000

     M49

    COMMISSION DECISION of 22 March 2000

      L 74

    19

    23.3.2000

     M50

    COMMISSION DECISION of 29 September 2000

      L 260

    52

    14.10.2000

     M51

    COMMISSION DECISION of 26 January 2001

      L 43

    38

    14.2.2001

     M52

    COMMISSION DECISION of 16 October 2001

      L 274

    22

    17.10.2001

     M53

    COMMISSION DECISION of 6 January 2004

      L 17

    41

    24.1.2004

    ►M54

    COMMISSION DECISION of 6 January 2004

      L 73

    11

    11.3.2004

    ►M55

    COMMISSION DECISION of 13 April 2004

      L 118

    45

    23.4.2004


    Amended by:

     A1

    Act of Accession of Austria, Sweden and Finland

      C 241

    21

    29.8.1994

     

    (adapted by Council Decision 95/1/EC, Euratom, ECSC)

      L 001

    1

    ..

     A2

    Act concerning the conditions of accession of the Czech Republic, the Republic of Estonia, the Republic of Cyprus, the Republic of Latvia, the Republic of Lithuania, the Republic of Hungary, the Republic of Malta, the Republic of Poland, the Republic of Slovenia and the Slovak Republic and the adjustments to the Treaties on which the European Union is founded

      L 236

    33

    23.9.2003


    Corrected by:

     C1

    Corrigendum, OJ L 039, 11.2.2004, p. 23  (81/04)




    ▼B

    ▼M54

    COUNCIL DECISION

    of 21 December 1976

    drawing up a list of third countries or parts of third countries, and laying down animal and public health and veterinary certification conditions, for importation into the Community of certain live animals and their fresh meat

    (79/542/EEC)

    ▼B



    THE COUNCIL OF THE EUROPEAN COMMUNITIES,

    Having regard to the Treaty establishing the European Economic Community,

    Having regard to Council Directive 72/462/EEC of 12 December 1972 on health and veterinary inspection problems upon importation of bovine animals and swine and fresh meat from third countries ( 1 ), as last amended by Directive 77/98/EEC ( 2 ), and in particular Article 3 (1) thereof,

    Having regard to the proposal from the Commission,

    Whereas the system laid down in Directive 72/462/EEC is based on the establishment of a list of the third countries or parts of third countries from which the Member States authorize imports of bovine animals and swine and of fresh meat of bovine animals, swine, sheep, goats and domestic solipeds, or of one or more of these categories of animals or categories of fresh meat;

    Whereas in order to decide in respect both of the animals and of fresh meat whether a country or part of a country may be included in the list, particular account is taken of the criteria set out in Article 3 (2) of the abovementioned Directive;

    Whereas the countries listed in the Annex to this Decision which traditionally supply the Member States may be considered to satisfy these criteria;

    Whereas, however, this list is drawn up subject to such amendments or additions as may be made to it in accordance with the procedure laid down in Article 30 of Directive 72/462/EEC; whereas it may prove necessary in the light of further information to limit or extend the authorizations for importing certain categories of animals and fresh meat; whereas, it may also be necessary in certain cases in respect both of the animals and of fresh meat to specify the parts of countries from which imports will be authorized;

    Whereas, although the list of third countries forms one of the bases of the Community arrangements applicable to imports from third countries laid down in Directive 72/462/EEC other measures, particularly concerning hygiene and veterinary inspection, will have to be taken in order to define these arrangements; whereas, consequently, it is important to facilitate the coordinated implementation of all these measures,

    HAS ADOPTED THIS DECISION:



    ▼M54

    Article 1

    Subject matter and scope

    This Decision establishes the sanitary conditions for the importation into the Community of live animals excluding equidae, and for the importation of fresh meat and meat products of such animals, including equidae, but excluding meat preparations.

    This Decision shall not apply to imports of non-domesticated animals for shows or exhibitions where such animals are not regularly kept or bred, and those non-domesticated animals forming part of circuses, or intended for scientific including conservation or experimental purposes in a body, institute or centre that has been approved in accordance with Annex C to Directive 92/65/EEC.

    Imports of animals and fresh meat authorised in accordance with this Decision shall remain subject to other provisions that have been adopted, or may be adopted, under European food law.

    Article 2

    Definitions

    For the purposes of this Decision, the following definitions shall apply:

    (a) ‘animals’: means land mammals of the species belonging to the taxa Proboscidea and Artiodactyla, and their crossbreeds;

    (b) ‘holding’: means a farm or other officially supervised agricultural, industrial or commercial undertaking, including zoos, amusement parks and wildlife or hunting reserves where animals are regularly kept or bred;

    (c) ‘trimmed offal’: means offal from which the bones, the cartilage, the trachea and main bronchi, the lymphatic glands and adhering connective tissue, the fat and the mucus have been completely removed; in the case of meat from domestic bovine animals, the whole masseter muscles, incised in accordance with point 41(a) of Chapter VIII of Annex I to Council Directive 64/433/EEC, are also considered as trimmed offal.

    Article 3

    Conditions for importation of live animals into the Community

    Imports into the Community of live animals shall only be allowed if such animals comply with Articles 4, 5 and 6.

    Article 4

    Place of origin of live animals

    The animals shall come from the territory of a third country or a part thereof as listed in columns 1, 2 and 3 of the table set out in Part 1 of Annex I for which, in the corresponding column 4, there is a specific model of veterinary certificate designated for these animals.

    Article 5

    Specific conditions

    The animals shall meet the requirements set out in the appropriate certificate established in accordance with the corresponding model certificate drawn up under Part 2 of Annex I, taking into account the specific conditions indicated in column 6 of the table set out in Part 1 of Annex I, and, if so indicated in column 5 of the table, they shall also meet any supplementary guarantees required in that certificate.

    If required by the Member State of destination, the animals concerned shall meet the additional certification requirements mentioned for that Member State and included in the certificate, based on the corresponding model set out in Part 2.

    Article 6

    Transport of live animals for importation into the Community

    1.  The animals shall not be loaded in a means of transport carrying other animals that are not destined for the Community or are of a lower health status.

    2.  During the transport to the Community, the animals shall not be unloaded in the territory of a third country or part of a third country that is not approved for importation into the Community of such animals.

    3.  During the transport to the Community, the animals shall not be moved by road, railway or on foot through the territory or part of the territory of a third country that is not approved for importation into the Community of such animals.

    4.  The animals shall arrive at a border inspection post of the Community within 10 days of the date of loading in the exporting third country and be accompanied by a veterinary certificate, drawn up in conformity with the corresponding model, completed and signed by an official veterinarian of the exporting third country.

    In the case of transport by sea, the period of 10 days shall be prolonged by the time of the sea journey. For that purpose, a declaration by the master of the ship, drawn up in accordance with the addendum of Part 3A of Annex I, shall be attached in its original form to the veterinary certificate.

    Article 7

    Conditions to be applied following importation

    Following the importation and in accordance with Directive 91/496/EEC,

    (i) animals intended for immediate slaughter shall be conveyed without delay to the slaughterhouse of destination where they shall be slaughtered within five working days;

    (ii) animals intended for breeding, production or fattening purposes, and animals intended for zoos, amusement parks and hunting or wildlife reserves, shall be conveyed without delay to the holding of destination where they shall remain for a minimum period of 30 days before further movement outside the holding, except in the case of direct dispatch to a slaughterhouse.

    Article 8

    Conditions for importation of fresh meat into the Community

    Imports into the Community of fresh meat intended for human consumption, from the animals as defined in Article 2 and from equidae, shall only be allowed if such meat complies with Articles 9 to 11.

    Article 9

    Place of origin of fresh meat

    The fresh meat shall come from the territory of a third country or a part thereof as listed in columns 1, 2 and 3 of the table set out in Part 1 of Annex II for which, in the corresponding column 4, there is a specific model of veterinary certificate designated for that meat.

    Article 10

    Specific conditions

    The fresh meat shall meet the requirements set out in the appropriate certificate corresponding to the model certificate drawn up under Part 2 of Annex II, taking into account the specific conditions indicated in column 6 of the table set out in Part 1 of Annex II, and, if so indicated in column 5 of the table, it shall also meet the supplementary guarantees requested in that certificate.

    Article 11

    Presentation of fresh meat at a Community border inspection post

    The fresh meat shall be presented at a Community border inspection post accompanied by a veterinary certificate, drawn up in conformity with the corresponding model, completed and signed by an official veterinarian of the exporting third country.

    Article 12

    Conditions to be applied following importation

    1.  Following importation, the following categories of fresh meat shall be conveyed without delay to the processing establishment of destination, in accordance with Directive 97/78/EC:

    (a) unskinned carcases of wild cloven-hoofed game intended for human consumption after further processing;

    (b) trimmed offal of domestic bovine animals intended for human consumption as meat-based products after further heat-treatment by cooking to a core temperature of at least 80 °C, or sterilised in hermetically sealed containers in a way as to achieve a value of Fo ≥ 3.

    2.  For the categories of products referred to in paragraph 1(b), the establishment of destination shall be an establishment specifically approved and registered for processing those products by the Member State in which the establishment is situated.

    3.  In accordance with the procedures established by Decision 2001/106/EC, Member States shall communicate to each other and to the Commission:

    (a) the names and addresses of the establishments referred to in paragraph 2 and of the local competent authority responsible for the supervision of these establishments, as well as

    (b) the categories of products for which these establishments are approved and registered.

    ▼M55

    Article 12b

    1.  By way of derogation from Article 12a, Member States shall authorise the transit by road or by rail through the Community, between the designated Community border inspection posts listed in Annex IV, of consignments coming from and destined to Russia directly or via another third country provided that the following conditions are met:

    (a) the consignment shall be sealed with a serially numbered seal at the border inspection post (BIP) of entry to the Community by the veterinary services of the competent authority;

    (b) the documents accompanying the consignment and referred to in Article 7 of Directive 97/78/EC shall be stamped ‘ONLY FOR TRANSIT TO RUSSIA VIA THE EC’ on each page by the official veterinarian of the competent authority responsible for the BIP;

    (c) the procedural requirements provided for in Article 11 of Directive 97/78/EC shall be complied with;

    (d) the consignment is certified as acceptable for transit on the common veterinary entry document by the official veterinarian of the border inspection post of introduction.

    2.  Unloading or storage, as defined in Article 12(4) or Article 13 of Directive 97/78/EC, of such consignments on Community territory shall not be allowed.

    3.  Regular audits shall be made by the competent authority to ensure that the number of consignments and the quantities of products leaving the Community territory matches the number and quantities entering.

    ▼M54

    Article 13

    Certification

    The veterinary certificates required for the importation of live animals and fresh meat into the Community, as provided for in this Decision, shall be drafted in accordance with the notes set out in Part 2 of Annexes I and II. However, this shall not preclude the use of electronic certification or other agreed systems, harmonised at Community level.

    ▼B

    Article  ►M54  14 ◄

    This Decision is addressed to the Member States.

    ▼M54




    ANNEX I (LIVE ANIMALS)

    PART 1

    List of third countries or parts thereof



    Country

    Code of territory

    Description of territory

    Veterinary certificate

    Specific conditions

    Model(s)

    SG

    1

    2

    3

    4

    5

    6

    BG — Bulgaria

    BG-0

    Whole country

    -

     

    VI

    BG-1

    The provinces of Varna, Dobrich, Silistra, Choumen, Targovitchte, Razgrad, Rousse, V.Tarnovo, Gabrovo, Pleven, Lovetch, Plovdic, Smolian, Pasardjik, Sofia district, Sofia city, Pernik, Kustendil, Blagoevgrad, Sliven, Starazagora, Vratza, Montana and Vidin

    BOV-X, BOV-Y, RUM, OVI-X, OVI-Y

    A

    CA — Canada

    CA-0

    Whole country

    POR-X

     

    IVb

    IX

    CA-1

    Whole country except the Okanagan Valley region of British Columbia, described as follows:

    — from a point on the Canada/United States border 120°15′ longitude, 49° latitude

    — northerly to a point 119°35′ longitude, 50°30′ latitude

    — north-easterly to a point 119° longitude, 50°45′ latitude

    — southerly to a point on the Canada/United States border 118°15′ longitude, 49° latitude

    BOV-X,

    OVI-X, OVI-Y

    A

    CH — Switzerland

    CH-0

    Whole country

    BOV-X, BOV-Y

    OVI-X, OVI-Y

    RUM

     
     

    POR-X, POR-Y

    SUI

    B

     

    CL — Chile

    CL-0

    Whole country

    OVI-X, RUM

     
     

    POR-X, SUI

    B

     

    CY — Cyprus

    CY-0

    Whole country

    POR-X, POR-Y

    B

     

    CZ — Czech Republic

    CZ-0

    Whole country

    BOV-X, BOV-Y, RUM, OVI-X, OVI-Y

    POR-X, POR-Y

     

    IVa

    V

    EE — Estonia

    EE-0

    Whole country

    BOV-X, BOV-Y, RUM, OVI-Y

     
     

    GL — Greenland

    GL-0

    Whole country

    OVI-X, RUM

     
     

    HR — Croatia

    HR-0

    Whole country

    BOV-X, BOV-Y, RUM, OVI-X, OVI-Y

     
     

    HU — Hungary

    HU-0

    Whole country

    BOV-X, BOV-Y, RUM,

    OVI-X, OVI-Y

    POR-X, POR-Y

    B

    V

    IS — Iceland

    IS-0

    Whole country

    BOV-X, BOV-Y

    RUM,

    OVI-X, OVI-Y

     

    I

    POR-X, POR-Y

    B

    LT — Lithuania

    LT-0

    Whole country

    BOV-X, BOV-Y

    OVI-Y, RUM

     
     

    LV — Latvia

    LV-0

    Whole country

    BOV-X, BOV-Y

    OVI-Y, RUM

     
     

    MT — Malta

    MT-0

    Whole country

    RUM, OVI-X, OVI-Y

     
     

    NZ — New Zealand

    NZ-0

    Whole country

    BOV-X, BOV-Y, RUM,

    POR-X, POR-Y

    OVI-X, OVI-Y

     

    I

    PL — Poland

    PL-0

    Whole country

    BOV-X, BOV-Y, RUM,

    OVI-X, OVI-Y

     
     

    PM — St Pierre Miquelon

    PM-0

    Whole country

     
     
     

    RO — Romania

    RO-0

    Whole country

    BOV-X, BOV-Y, RUM,

    OVI-X, OVI-Y

     

    V

    SI — Slovenia

    SI-0

    Whole country

    BOV-X, BOV-Y, RUM,

    OVI-Y

     
     

    SK — Slovakia

    SK-0

    Whole country

    BOV-X, BOV-Y, RUM,

    OVI-X, OVI-Y

     

    V

    Specific conditions (see footnotes in each certificate):

    ‘I’

    :

    territory where the presence of BSE in native cattle has been assessed as highly unlikely, for the purpose of exporting to the European Community animals certified according to the models of certificate BOV-X and BOV-Y.

    ‘II’

    :

    territory recognised as having an official tuberculosis-free status for the purposes of exports to the European Community of animals certified according to the model of certificate BOV-X.

    ‘III’

    :

    territory recognised as having an official brucellosis-free status for the purposes of exports to the European Community of animals certified according to the model of certificate BOV-X.

    ‘IVa’

    :

    territory recognised as having an official enzootic-bovine-leukosis (EBL) free status for the purposes of exports to the European Community of animals certified according to the model of certificate BOV-X.

    ‘IVb’

    :

    territory with approved holdings recognised as having an official enzootic-bovine-leukosis (EBL) free status for the purposes of exports to the European Community of animals certified according to the model of certificate BOV-X.

    ‘V’

    :

    territory recognised as having an official brucellosis-free status for the purposes of exports to the European Community of animals certified according to the model of certificate OVI-X.

    ‘VI’

    :

    Geographical constraints:

    In the case of Bulgaria, code of territory BG-1, animals certified according to models of veterinary certificate BOV-X, BOV-Y, RUM, OVI-X and OVI-Y can be imported only in those parts of the territory of a Member State appearing in Annex II to Decision 2001/138/EC of 9 February 2001, if that Member State so allows.

    ‘VII’

    :

    territory recognised as having an official tuberculosis-free status for the purposes of exports to the European Community of animals certified according to the model of certificate RUM.

    ‘VIII’

    :

    territory recognised as having an official brucellosis-free status for the purposes of exports to the European Community of animals certified according to the model of certificate RUM.

    ‘IX’

    :

    territory recognised as having an official Aujeszky's disease-free status for the purposes of exports to the European Community of animals certified according to the model of certificate POR-X.

    PART 2

    Models of veterinary certificates

    Models:

    ‘BOV-X’

    :

    Model of veterinary certificate for domestic bovine animals (Bos taurus, Bison bison, Bubalus bubalis and their cross-breeds) intended for breeding and/or production after importation

    ‘BOV-Y’

    :

    Model of veterinary certificate for domestic bovine animals (Bos taurus, Bison bison, Bubalus bubalis and their cross-breeds) intended for immediate slaughter after importation

    ‘OVI-X’

    :

    Model of veterinary certificate for domestic sheep (Ovis aries) and goats (Capra hircus) intended for breeding and/or production after importation

    ‘OVI-Y’

    :

    Model of veterinary certificate for domestic sheep (Ovis aries) and goats (Capra hircus) intended for immediate slaughter after importation

    ‘POR-X’

    :

    Model of veterinary certificate for domestic porcine animals (Sus scrofa) intended for breeding and/or production after importation

    ‘POR-Y’

    :

    Model of veterinary certificate for domestic porcine animals (Sus scrofa) intended for immediate slaughter after importation

    ‘RUM’

    :

    Model of veterinary certificate for non-domestic animals other than suidae

    ‘SUI’

    :

    Model of veterinary certificate for non-domestic suidae.

    SG (supplementary guarantees):

    ‘A’

    :

    guarantees regarding bluetongue and epizootic-haemorrhagic disease tests on animals certified according to the model of certificate BOV-X (point 10.8a), OVI-X (point 10.6a) and RUM (point 10.7a)

    ‘B’

    :

    guarantees regarding swine-vesicular disease and classical-swine-fever tests on animals certified according to the model of certificate POR-X (point 10.4a) and SUI (point 10.4a)

    ‘C’

    :

    guarantees regarding brucellosis test on animals certified according to the model of certificate POR-X (point 10.4a) and SUI (point 10.4a)

    Notes

    (a) Veterinary certificates shall be produced by the exporting country, based on the models appearing in Part 2 of Annex I, according to the layout of the model that corresponds to the animals concerned. They shall contain, in the numbered order that appears in the model, the attestations that are required for any third country and, as the case may be, those supplementary guarantees that are required for the exporting third country or part thereof.

    If so requested by the EU Member State of destination, for the animals concerned the additional certification requirements shall be also incorporated in the original form of the veterinary certificate.

    (b) A separate and unique certificate must be provided for animals that are exported from a single territory appearing in columns 2 and 3 of Part 1 of Annex I which are consigned to the same destination and transported in the same railway wagon, lorry, aircraft or ship.

    (c) The original of each certificate shall consist of a single page, both sides, or, where more text is required, it shall be in such a form that all pages needed are part of an integrated whole and indivisible.

    (d) It shall be drawn up in at least one of the official languages of the EU Member State in which the inspection at the border post shall be carried out and of the EU Member State of destination. However, these Member States may allow another Community language instead of their own, accompanied, if necessary, by an official translation.

    (e) If for reasons of identification of the items of the consignment (schedule in point 8.2 of the model of certificate), additional pages are attached to the certificate, these pages shall also be considered as forming part of the original of the certificate by the application of the signature and stamp of the certifying official veterinarian on each of the pages.

    (f) When the certificate, including additional schedules referred to in (e), comprises more than one page, each page shall be numbered — (page number) of (total number of pages) — at the bottom and shall bear the code number of the certificate that has been designated by the competent authority at the top.

    (g) The original of the certificate must be completed and signed by an official veterinarian within 24 hours prior to loading of the consignment for exportation to the Community. In doing so, the competent authorities of the exporting country shall ensure that principles of certification equivalent to those laid down in Council Directive 96/93/EC are followed.

    The colour of the signature shall be different to that of the printing. The same rule applies to stamps other than those embossed or watermark.

    (h) The original of the certificate must accompany the consignment until it reaches the EU border inspection post.

    (i) The certificate shall be valid for 10 days from the date of issuing.

    In the case of transport by ship the time of validity is prolonged by the time of the trip in the ship. For this purpose, a declaration by the master of the ship, drawn up in accordance with the addendum to Part 3 of Annex I to this Decision, shall be attached in its original form to the veterinary certificate.

    (j) Animals shall not be transported together with other animals that either are not destined to the European Community or are of a lower health status.

    (k) During their transport to the European Community, the animals shall not be unloaded in the territory of a country or part of a country that is not approved for imports into the Community of these animals.

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    PART 3

    A —   Addendum for transport of animals by sea

    (To be completed and attached to the veterinary certificate when transport to the European Community frontier includes, even for part of the journey, transportation by ship.)

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    B —   Conditions for the authorisation of assembly centres

    Approved assembly centres shall meet the following requirements:

    I. They shall be supervised by an official veterinarian.

    II. They shall each be situated at the centre of an area 20 km in diameter in which, according to official findings, for at least 30 days prior to their use as approved centres there has been no case of foot-and-mouth disease.

    III. They shall, before each use as approved centres, be cleaned and disinfected with a disinfectant officially authorised in the exporting country as effective in the control of the disease mentioned in condition II above.

    IV. They shall have, taking into account their animal capacity (a) a facility dedicated exclusively for this purpose; (b) appropriate facilities, easy to clean and disinfect, for loading, unloading and adequate housing of a suitable standard for the animals, for watering and feeding them, and for giving them any necessary treatment; (c) appropriate facilities for inspection and isolation; (d) appropriate equipment for cleaning and disinfecting rooms and trucks; (e) an appropriate storage area for fodder, litter and manure; (f) appropriate systems for collecting and disposal of waste water; (g) an office for the official veterinarian.

    V. When operating, they shall have sufficient veterinarians to carry out all duties.

    VI. They shall only admit animals that are individually identified so as to guarantee traceability. To this end, when animals are admitted the owner or person in charge of the centre shall ensure the animals are properly identified and accompanied by health documents or certificates for the species and categories involved. Moreover, this person shall record on a register or a database and retain for at least three years the name of the owner, the origin, date of entry and exit, number and identification of the animals or registration number of the herd of origin and their destination and the registration number of the carrier and the registration number of the lorry delivering or collecting animals from the premises.

    VII. All animals passing through them shall fulfil the health conditions established for the importation of the relevant category of animal into the European Community.

    VIII. Animals to be exported to the European Community which pass through an assembly centre must, within six days of arrival, be loaded and dispatched directly to the frontier of the exporting country: (a) without coming into contact with cloven-hoofed animals other than animals which fulfil the health conditions established for the importation of the relevant category of animal into the European Community; (b) segregated into consignments so that no consignment contains both animals for breeding or production and animals for immediate slaughter; (c) in transport vehicles or containers which have first been cleaned and disinfected with a disinfectant officially authorised in the exporting country as effective in the control of the disease mentioned in condition II above and which are so constructed that faeces, urine, litter or fodder cannot flow or fall out during transportation.

    IX. Where the conditions for the export of animals to the Community require that a test be carried out within a specified period before loading, that period includes any period of assembly, up to six days, after the arrival of the animals at the approved centres.

    X. The exporting country shall designate those approved centres which are approved for animals for breeding and production and those approved centres which are approved for animals for slaughter and shall notify the Commission and the competent central authorities of the Member States of the names and addresses of such premises and their regular updates.

    XI. The exporting country shall determine the procedure for official supervision of approved centres and shall ensure that such supervision is carried out.

    XII. They shall be regularly inspected in order to ascertain that the requirements for approval continue to be fulfilled. In case of failure and suspension, the approval may only be restored when the competent authority is satisfied the full compliance of the centre with all the provisions mentioned above.

    C —   Protocols for the standardisation of materials and testing procedures

    Tuberculosis (TBL)

    The single intradermal tuberculin test using bovine tuberculin shall be carried out according to Annex B to Directive 64/432/EEC. In the case of Suidae animals, the single intradermal tuberculin test using avian tuberculin shall be carried out according to Annex B to 64/432/EEC, except that the site of injection shall be the loose skin at the base of the ear.

    Brucellosis (Brucella abortus) (BRL)

    The serum agglutination test, complement fixation test, buffered brucella antigen test and enzyme linked immuno-absorbent assays tests (ELISA) shall be carried out according to Annex C to Directive 64/432/EEC.

    Brucellosis (Brucella melitensis) (BRL)

    Test shall be carried out according to Annex C to Directive 91/68/EEC.

    Enzootic Bovine Leukosis (EBL)

    The agar gel immuno-diffusion test and the enzyme linked immuno-absorbent assay test (ELISA) shall be carried out according to paragraphs A and C, chapter II of Annex D to Council Directive 64/432/EEC.

    Bluetongue (BTG)

    A. The blocking or competitive ELISA test shall be carried out according to the following protocol:

    The competitive ELISA using monoclonal antibody 3-17-A3 is capable of identifying antibodies to all known serotypes of bluetongue virus (BTV).

    The principle of the test is the interruption of the reaction between BTV antigen and a group-specific monoclonal antibody (3-17-A3) by the addition of test serum. Antibodies to BTV present in the test serum block the reactivity of the monoclonal antibody (Mab) and result in a reduction in the expected colour development after the addition of enzyme labelled anti-mouse antibody and chromogen/substrate. Sera can be tested at a single dilution of 1:5 (spot test — appendix 1) or may be titrated (serum titration — appendix 2) to give dilution end-point. Inhibition values higher than 50 % may be regarded as positive.

    Material and reagents:

    1. Appropriate ELISA microtitre plates.

    2. Antigen: supplied as a cell extracted concentrate, prepared as described below, and stored at either -20 °C or -70 °C.

    3. Blocking buffer: phosphate buffered saline (PBS) containing 0,3 % BTV negative adult bovine serum, 0,1 % (v/v) Tween-20 (supplied as polyoxyethylene sorbiton monolaurate syrup) in PBS.

    4. Monoclonal antibody: 3-17-A3 (supplied as hybridoma tissue-culture supernatant) directed against the group-specific polypeptide VP7, stored at -20 °C or freeze-dried and diluted 1/100 with blocking buffer before use.

    5. Conjugate: rabbit anti-mouse globulin (adsorbed and eluted) conjugated to horseradish peroxidase and kept in the dark at 4 °C.

    6. Chromogen and substrate: Orthophenylene diamine (OPD-chromogen) at a final concentration of 0,4 mg/ml in sterile distilled water. Hydrogen peroxide (30 % w/v-substrate) 0,05 % v/v added immediately before use (5μl H2O2 per 10 ml OPD). (Handle OPD with care — wear rubber gloves — suspected mutagen).

    7. 1 Molar sulphuric acid: 26,6 ml of acid added to 473,4 ml of distilled water. (Remember — always add acid to water, never water to acid.)

    8. Orbital shaker.

    9. ELISA plate reader (the test may be read visually).

    Test format

    Cc: conjugate control (no serum/ no monoclonal antibody); C++: strong positive serum control; C+: weak positive serum control; C-: negative serum control; Cm: monoclonal antibody control (no serum).



    Appendix 1: Spot dilution (1:5) format (40 sera/plate)

     

    Controls

    Test sera

     

    1

    2

    3

    4

    5

    6

    7

    8

    9

    10

    11

    12

    A

    Cc

    C-

    1

    2

    3

    4

    5

    6

    7

    8

    9

    10

    B

    Cc

    C-

    1

    2

    3

    4

    5

    6

    7

    8

    9

    10

    C

    C++

    C++

     
     
     
     
     
     
     
     
     
     

    D

    C++

    C++

     
     
     
     
     
     
     
     
     
     

    E

    C+

    C+

     
     
     
     
     
     
     
     
     
     

    F

    C+

    C+

     
     
     
     
     
     
     
     
     
     

    G

    Cm

    Cm

     
     
     
     
     
     
     
     
     

    40

    H

    Cm

    Cm

     
     
     
     
     
     
     
     
     

    40



    Appendix 2: Serum titration format (10 sera/plate)

     

    Controls

    Test sera

     

    1

    2

    3

    4

    5

    6

    7

    8

    9

    10

    11

    12

    A

    Cc

    C-

    1:5

     
     
     
     
     
     
     
     

    1:5

    B

    Cc

    C-

    1:10

     
     
     
     
     
     
     
     

    1:10

    C

    C++

    C++

    1:20

     
     
     
     
     
     
     
     

    1:20

    D

    C++

    C++

    1:40

     
     
     
     
     
     
     
     

    1:40

    E

    C+

    C+

    1:80

     
     
     
     
     
     
     
     

    1:80

    F

    C+

    C+

    1:160

     
     
     
     
     
     
     
     

    1:160

    G

    Cm

    Cm

    1:320

     
     
     
     
     
     
     
     

    1:320

    H

    Cm

    Cm

    1:640

     
     
     
     
     
     
     
     

    1:640

    Test protocol:

    Conjugate control (Cc) : Wells 1A and 1B is a blank control consisting of BTV antigen and conjugate. This may be used to blank the ELISA reader.

    Mab control (Cm) : Columns 1 and 2, rows G and H are the monoclonal antibody control and contain BTV antigen, monoclonal antibody and conjugate. These wells represent maximum colour. The mean of the optical density readings from this control represents the 0 % inhibition value.

    Positive control (C++, C-) : Columns 1 and 2, rows C-D-E-F. These wells contain BTV antigen, BTV strong and weak positive antiserum respectively, Mab and conjugate.

    Negative control (C-) : Wells 2A and 2B are the negative controls, which contain BTV antigen, BTV negative antiserum, Mab and conjugate.

    Test sera : For large-scale serological surveys and rapid screening, sera could be tested at a single dilution of 1:5 (Appendix 1). Alternatively, 10 sera can be tested over a dilution range from 1:5 to 1:640 (Appendix 2). This will give some indication of the titre of antibody in the test sera.

    Procedure:

    1. Dilute BTV antigen to pre-titrated concentration in PBS, sonicate briefly to disperse aggregated virus (if sonicator is not available, pipette vigorously) and add 50 μl to all wells of the ELISA plate. Tap sides of plate to disperse antigen.

    2. Incubate at 37 °C for 60 minutes on an orbital shaker. Wash plates three times by flooding and emptying the wells with non-sterile PBS and blot dry on absorbent paper.

    3. Control wells: Add 100 μl of blocking buffer to Cc wells. Add 50 μl of positive and negative control sera, at a dilution of 1:5 (10 μl sera + 40 μl blocking buffer), to respective wells C-, C+ and C++. Add 50 μl blocking buffer to Mab control wells.

    Spot titration method: Add a 1:5 dilution of each test serum in blocking buffer to duplicate wells of columns 3 to 12 (10 μl sera + 40 μl blocking buffer),

    or

    Serum titration method: Prepare a two-fold dilution series of each test sample (1:5 to 1:640) in blocking buffer across eight wells of single columns 3 to 12.

    4. Immediately after the addition of the test sera, dilute Mab 1:100 in blocking buffer and add 50 μl to all wells of the plate except for the blank control.

    5. Incubate at 37 °C for 60 minutes on an orbital shaker. Wash three times with PBS and blot dry.

    6. Dilute rabbit anti-mouse concentrate to 1/5 000 in blocking buffer and add 50 μl to all wells of the plate.

    7. Incubate at 37 °C for 60 minutes on an orbital shaker. Wash three times with PBS and blot dry.

    8. Thaw the OPD and immediately before use add 5 μl of 30 % hydrogen peroxide to each 10 ml of OPD. Add 50 μl to all wells of the plate. Allow colour to develop for approximately 10 minutes and stop the reaction with 1 M sulphuric acid (50 μl per well). Colour should develop in the Mab control wells and in those wells containing sera with no antibody to BTV.

    9. Examine and record the plates either visually or using a spectrophotometric reader.

    Analysis of results:

    Using the software package print out the OD values, and the percentage inhibition (PI) for test and control sera based on the mean value recorded in the antigen control wells. The date expressed as OD and PI values are used to determine whether the test has performed within acceptable limits. The upper control limits (UCL) and lower control limits (LCL) for the Mab control (antigen plus Mab in the absence of test sera) are between OD values 0,4 and 1,4. Any plate that fails to conform to the above criteria must be rejected.

    If a computer software package is not available, print out the OD values using the ELISA printer. Calculate the mean OD value for the antigen control wells, which is equivalent to the 100 % value. Determine the 50 % OD value and manually calculate the positivity and negativity of each sample.

    Percentage inhibition (PI) value = 100 — (OD of each test control/Mean OD of Cm) × 100.

    The duplicate negative control serum wells and the duplicate blank wells should record PI values between +25 % and -25 %, and between +95 % and +105 %, respectively. Failure to be within these limits does not invalidate the plate but does suggest that background colour is developing. The strong and weak positive control sera should record PI values between +81 % and +100 %, and between +51 % and +80 %, respectively.

    The diagnostic threshold for test sera is 50 % (PI 50 % or OD 50 %). Samples recording PI values > 50 % are recorded negative. Samples that record PI values above and below the threshold for the duplicate wells are considered doubtful; such samples may be retested in the spot test and/or titration. Positive samples may also be titrated to provide an indication of the degree of positivity.

    Visual reading: Positive and negative samples are easily discernible by eye; weakly positive or strong negative samples may be more difficult to interpret by eye.

    Preparation of BTV ELISA antigen:

    1. Wash 40-60 roux of confluent BHK-21 cells three times with serum-free Eagle's medium and infect with bluetongue virus serotype 1 in serum-free Eagle's medium.

    2. Incubate at 37 °C and examine daily for cytopathic effect (CPE).

    3. When CPE are complete in 90 to 100 % of the cell sheet of each roux, harvest the virus by shaking any still-attached cells from the glass.

    4. Centrifuge at 2 000 to 3 000 rpm to pellet the cells.

    5. Discard the supernatant and re-suspend the cells in approximately 30 ml of PBS containing 1 % ‘Sarkosyl’ and 2 ml phenylmethylsulphonyl fluoride (lysis buffer). This may cause the cells to form a gel and more lysis buffer may be added to reduce this effect. (NB: phenylmethylsulphonyl fluoride is harmful — handle with extreme caution.)

    6. Disrupt the cells for 60 seconds using an ultrasonic probe at an amplitude of 30 microns.

    7. Centrifuge at 10 000 rpm for 10 minutes.

    8. Store the supernatant at +4 °C and resuspend the remaining cell pellet in 10 to 20 ml of lysis buffer.

    9. Sonicate and clarify, storing the supernatant at each stage, a total of three times.

    10. Pool the supernatants and centrifuge at 24 000 rpm (100 000 g) for 120 minutes at +4 °C over a 5 ml cushion of 40 % sucrose (w/v in PBS) using 30 ml Beckmann centrifuge tubes and an SW 28 rotor.

    11. Discard the supernatant, drain the tubes thoroughly and re-suspend the pellet in PBS by sonication. Store the antigen in aliquots at -20 °C.

    Titration of BTV ELISA antigen:

    Bluetongue ELISA antigen is titrated by the indirect ELISA. Twofold dilutions of antigen are titrated against a constant dilution (1/100) monoclonal antibody 3-17-A3. The protocol is as follows:

    1. Titrate a 1:20 dilution of BTV antigen in PBS across the microtitre plate in a twofold dilution series (50 μl/well) using a multichannel pipette.

    2. Incubate for one hour at 37 °C on an orbital shaker.

    3. Wash plates three times with PBS.

    4. Add 50 μl of monoclonal antibody 3-17-A3 (diluted 1/100) to each well of the microtitre plate.

    5. Incubate for one hour at 37 °C on an orbital shaker.

    6. Wash plates three times with PBS.

    7. Add 50 μl of rabbit anti-mouse globulin conjugated to horseradish peroxidase, diluted to a pretitrated optimal concentration, to each well of the microtitre plate.

    8. Incubate for one hour at 37 °C on an orbital shaker.

    9. Add substrate and chromogen as described previously. Stop the reaction after 10 minutes by the addition of 1 Molar sulphuric acid (50 μl/well).

    In the competitive assay, the monoclonal antibody must be in excess, therefore a dilution of antigen is chosen which falls on the titration curve (not on the plateau region) which gives approximately 0,8 OD after 10 minutes.

    B. The agar gel immuno-diffusion test shall be carried out according to the following protocol:

    Antigen:

    Precipitating antigen is prepared in any cell culture system that supports the rapid multiplication of a reference strain of bluetongue virus. BHK or Vero cells are recommended. Antigen is present in the supernatant fluid at the end of virus growth but requires 50 to 100-fold concentration to be effective. This may be achieved by any standard protein concentration procedure; virus in the antigen may be inactivated by the addition of 0,3 % (v/v) beta-propiolactone.

    Known positive control serum:

    Using the international reference serum and antigen a national standard serum is produced, standardised for optimal proportion against the international reference serum, freeze-dried and used as the known control serum in each test.

    Test serum

    Procedure : 1 % agarose prepared in borate or sodium barbitol buffer, pH 8,5 to 9,0, is poured into a petri dish to a minimum depth of 3,0 mm. A test pattern of seven moisture-free wells, each 5,0 mm in diameter, is cut in the agar. The pattern consists of one centre well and six wells arranged round it in a circle of radius 3 cm. The central well is filled with the standard antigen. Peripheral wells 2, 4 and 6 are filled with known positive serum, wells 1, 3 and 5 are filled with test sera. The system is incubated for up to 72 hours at room temperature in a closed humid chamber.

    Interpretation : A test serum is positive if it forms a specific precipitin line with the antigen and forms a complete line of identity with the control serum. A test serum is negative if it does not form a specific line with the antigen and it does not bend the line of the control serum. Petri dishes should be examined against a dark background and using indirect illumination.

    Epizootic haemorrhagic disease (EHD)

    The agar gel immuno-diffusion test shall be carried out according to the following protocol:

    Antigen:

    Precipitating antigen is prepared in any cell culture system that supports the rapid multiplication of the appropriate serotype(s) of epizootic haemorrhagic disease virus. BHK or Vero cells are recommended. Antigen is present in the supernatant fluid at the end of virus growth but requires 50 to 100-fold concentration to be effective. This may be achieved by any standard protein concentration procedure; virus in the antigen may be inactivated by the addition of 0,3 % (v/v) beta-propiolactone.

    Known positive control serum:

    Using the international reference serum and antigen a national standard serum is produced, standardised for optimal proportion against the international reference serum, freeze-dried and used as the known control serum in each test.

    Test serum

    Procedure : 1 % agarose prepared in borate or sodium barbitol buffer, pH 8,5 to 9,0, is poured into a petri dish to a minimum depth of 3,0 mm. A test pattern of seven moisture-free wells, each 5,0 mm in diameter, is cut in the agar. The pattern consists of one centre well and six wells arranged round it in a circle of radius 3 cm. The central well is filled with the standard antigen. Peripheral wells 2, 4 and 6 are filled with known positive serum, wells 1, 3 and 5 are filled with test sera. The system is incubated for up to 72 hours at room temperature in a closed humid chamber.

    Interpretation : A test serum is positive if it forms a specific precipitin line with the antigen and forms a complete line of identity with the control serum. A test serum is negative if it does not form a specific line with the antigen and it does not bend the line of the control serum. Petri dishes should be examined against a dark background and using indirect illumination.

    Infectious bovine rhinotracheitis (IBR)/infectious pustular vulvo-vaginitis (IPV)

    A. The serum neutralisation test shall be carried out according to the following protocol:

    Serum : All sera are heat-inactivated at 56 °C for 30 minutes before use.

    Procedure : The constant virus-varying serum neutralisation test on microtitre plates employs MDBK or other susceptible cells. The Colorado, Oxford or any other reference strain of the virus is used at 100 TCID50 per 0,025 ml; inactivated undiluted serum samples are mixed with an equal volume (0,025 ml) of virus suspension. The virus/serum mixtures are incubated for 24 hours at 37 °C in the microtitre plates before the MDBK cells are added. Cells are used at a concentration which forms a complete monolayer after 24 hours.

    Controls : (i) virus infectivity assay, (ii) serum toxicity controls, (iii) uninoculated cell culture controls, (iv) reference antisera.

    Interpretation : The results of the neutralisation test and the titre of the virus used in the test are recorded after three to six days incubation at 37 °C. Serum titres are considered negative if there is no neutralisation at a dilution of 1/2 (undiluted serum).

    B. Any other test recognised in the frame of Commission Decision 93/42/EC concerning additional guarantees to infectious rhinotracheitis for bovines destined for Member States or regions thereof free from the disease.

    Foot-and-mouth disease (FMD)

    A. Collecting oesophageal/pharyngeal samples and testing shall be carried out according to the following protocol:

    Reagents : Prior to sampling, transport medium is prepared. Two ml volumes are dispensed in as many containers as there are animals to be sampled. The containers used should withstand freezing over solid CO2 or liquid nitrogen. Samples are obtained by the use of a specially-designed sputum collector or ‘probang’. To obtain a sample the probang cup is passed through the mouth, over the dorsum of the tongue and down into the upper part of the oesophagus. Attempts are made to scrape the surface epithelium of the upper oesophagus and pharynx by movements directed laterally and dorsally. The probang is then withdrawn, preferably after the animal has swallowed. The cup should be full and contain a mixture of mucus, saliva, oesophageal fluid and cellular debris. Care should be taken to ensure that each specimen contains some visible cellular material. Very rough handling which causes bleeding should be avoided. Samples from some animals may be heavily contaminated with ruminal contents. Such samples should be discarded and the mouth of the animal flushed with water, or preferably physiological saline, before repeat sampling.

    Treatment of samples : Each sample collected in the probang cup is examined for quality and 2 ml added to an equal volume of transport medium in a container which can withstand freezing. The containers are tightly closed, sealed, disinfected and labelled. The samples are kept cool (+4 °C) and examined within three to four hours or placed over dry ice (-69 °C) or liquid nitrogen and kept frozen until examined. Between animals the probang is disinfected and washed in three changes of clean water.

    Testing for FMD virus : Samples are inoculated into cultures of primary bovine thyroid cell cultures using at least three tubes per sample. Other susceptible cells e. g. primary bovine or porcine kidney cells can be used but it should be kept in mind that for some strains of FMD virus they are less sensitive. The tubes are incubated at 37 °C on a roller apparatus and examined daily for 48 hours for the presence of a cytopathic effect (CPE). If negative, cultures are blind passaged onto new cultures and re-examined for 48 hours. The specificity of any CPE must be confirmed.

    Recommended transport media:

    1. 0,08M phosphate buffer pH 7,2 containing 0,01 % bovine serum albumin, 0,002 % phenol red and antibiotics.

    2. Tissue culture medium (e.g. Eagle's MEM) containing 0,04M Hepes buffer, 0,01 % bovine serum albumin and antibiotics, pH 7,2.

    3. Antibiotics (per ml final) should be added to the transport medium, e.g. penicillin 1 000 IU, neomycin sulphate 100 IU, polymyxin B sulphate 50 IU, mycostatin 100 IU.

    B. The virus neutralisation test shall be carried out according to the following protocol:

    Reagents : Stock FMDV antigen is prepared in cell cultures or on cattle tongues and stored at -70 °C or less or at -20 °C after the addition of 50 % glycerol. This is the stock antigen. FMDV is stable under these conditions and titres vary little over a period of months.

    Procedure : The test is carried out in flat-bottomed tissue culture grade microtitre plates using susceptible cells such as IB-RS-2, BHK-21 or calf kidney cells. Sera for the test are diluted 1/4 in serum-free cell culture medium with the addition of 100 IU/ml neomycin or other suitable antibiotics. Sera are inactivated at 56 °C for 30 minutes and 0,05 ml amounts are used to prepare a twofold series on microtitre plates using 0,05 ml diluting loops. Pretitrated virus also diluted in serum-free culture medium and containing 100 TCID50/0,05 ml is then added to each well. Following incubation at 37 °C for one hour to allow neutralisation to take place, 0,05 ml of suspension cells containing 0,5 to 1,0 × 106 cells per 1 ml in cell culture medium containing serum free of FMD antibody is added to each well and the plates are sealed. Plates are incubated at 37 °C. Monolayers are normally confluent within 24 hours. CPE is usually sufficiently advanced at 48 hours for a microscopic reading of the test. At this time a final microscopic reading may be made or the plates may be fixed and stained for macroscopic reading, for instance using 10 % formol-saline and 0,05 % methylene blue.

    Controls : Controls in each test include homologous antiserum of known titre, a cell control, a serum toxicity control a medium control and a virus titration from which the actual amount of virus in the test is calculated.

    Interpretation : Wells with evidence of CPE are considered to be infected and neutralisation titres are expressed as the reciprocal of the final dilution of serum present in the serum/virus mixtures at the 50 % end point estimated according to the Spearman-Karber method. (Karber, G., 1931, Archiv fuer Experimentelle Pathologie und Pharmokologie, 162, 480). Tests are considered to be valid when the actual amount of virus used per well in the test is between 101,5 and 102,5 TCID50 and when the titre of the reference serum is within twofold of its expected titre, estimated from the mode of previous titrations. When the controls are outside these limits the tests are repeated. An end point titre of 1/11 or less is taken as negative.

    C. The detection and quantification of antibody by ELISA shall be carried out according to the following protocol:

    Reagents : Rabbit antisera to 146S antigen of seven types of foot-and-mouth disease virus (FMDV) used at a predetermined optimum concentration in carbonate/bicarbonate buffer, pH 9,6. Antigens are prepared from selected strains of virus grown on monolayers of BHK-21 cells. The unpurified supernatants are used and pretitrated according to the protocol but without serum, to give a dilution which after the addition of an equal volume of PBST (phosphate buffered saline containing 0,05 % Tween-20 and phenol red indicator) would give an optical density reading of between 1,2 and 1,5. The viruses can be used inactivated. PBST is used as a diluent. Guinea-pig antisera are prepared by inoculating guinea pigs with 146S antigen of each serotype. A predetermined optimum concentration is prepared in PBST containing 10 % normal bovine serum and 5 % normal rabbit serum. Rabbit anti-guinea-pig immunoglobulin conjugated to horseradish peroxidase is used at a predetermined optimum concentration in PBST containing 10 % normal bovine serum and 5 % normal rabbit serum. Test sera are diluted in PBST.

    Procedure:

    1. ELISA plates are coated with 50 μl of rabbit antiviral sera overnight in a humidity chamber at room temperature.

    2. Fifty microlitres of a duplicate, twofold series of each test serum starting at 1/4 are prepared in U-bottomed multiwell plates (carrier plates). Fifty microlitres of a constant dose of antigen are added to each well and the mixtures are left overnight at 4 °C. The addition of the antigen reduces the starting serum dilution to 1/8.

    3. The ELISA plates are washed five times with PBST.

    4. Fifty microlitres of serum/antigen mixtures are then transferred from the carrier plates to the rabbit-serum-coated ELISA plates and incubated at 37 °C for one hour on a rotary shaker.

    5. After washing, 50 μl of guinea-pig antiserum to the antigen used in point 4 is added to each well. The plates are incubated at 37 °C for one hour a rotary shaker.

    6. The plates are washed and 50 μl of rabbit anti-guinea-pig immunoglobulin conjugated to horseradish peroxidase is added to each well. The plates are incubated at 37 °C for one hour on a rotary shaker.

    7. The plates are washed and 50 μl of orthophenylene diamine containing 0,05 % H2O2 (30 %) w/v is added to each well.

    8. The reaction is stopped after 15 minutes with 1,25M H2SO4.

    The plates are read spectrophotometrically at 492 nm on an ELISA reader linked to a microcomputer.

    Controls : For each antigen used 40 wells contain no serum but contain antigen diluted in PBST. A duplicated twofold dilution series of homologous bovine reference antiserum. A duplicate twofold dilution series of negative bovine serum.

    Interpretation : Antibody titres are expressed as the final dilution of tests serum giving 50 % of the mean OD value recorded in the virus control wells where test serum is absent. Titres in excess of 1/40 are considered positive.

    References : Hamblin C, Barnett ITR and Hedger RS (1986) ‘A new enzyme-linked immunosorbent assay (ELISA) for the detection of antibodies against foot-and-mouth disease virus. I. Development and method of ELISA.’Journal of Immunological Methods, 93, 115 to 121.11.

    Aujeszky's disease (AJD)

    A. The serum neutralisation test shall be carried out according to the following protocol:

    Serum : All sera are heat-inactivated at 56 °C for 30 minutes before use.

    Procedure : The constant virus-varying serum neutralisation test on microtitre plates employs Vero or other sensitive cell systems. Aujeszky's disease virus is used at 100 TCID50 per 0,025 ml; inactivated undiluted serum samples are mixed with an equal volume (0,025 ml) of virus suspension. The virus/serum mixtures are incubated for two hours at 37 °C in the microtitre plates before the appropriate cells are added. Cells are used at a concentration which forms a complete monolayer after 24 hours.

    Controls : (i) virus infectivity assay, (ii) serum toxicity controls, (iii) uninoculated cell culture controls, (iv) reference antisera.

    Interpretation : The results of the neutralisation test and the titre of the virus used in the test are recorded after three to seven days incubation at 37 °C. Serum titres less than 1/2 (undiluted serum) are considered negative.

    B. Any other test recognised in the frame of Commission Decision 2001/618/EC concerning additional guarantees to Aujeszky's disease for pigs destined for certain parts of the territory of the Community.

    Transmissible gastroenteritis (TGE)

    The serum neutralisation test shall be carried out according to the following protocol:

    Serum : All sera are heat-inactivated at 56 °C for 30 minutes before use.

    Procedure : The constant virus-varying serum neutralisation test on microtitre plates employs A72 (dog tumour) cells or other sensitive cell systems. TGE virus is used at 100 TCID50 per 0,025 ml; inactivated undiluted serum samples are mixed with an equal volume (0,025 ml) of virus suspension. The virus/serum mixtures are incubated for 30 to 60 minutes at 37 °C in the microtitre plates before the appropriate cells are added. Cells are used at a concentration which forms a complete monolayer after 24 hours. Each cell receives 0,1 ml of cell suspension.

    Controls : (i) virus infectivity assay, (ii) serum toxicity controls, (iii) uninoculated cell culture controls, (iv) reference antisera.

    Interpretation : The results of the neutralisation test and the titre of the virus used in the test are recorded after three to five days incubation at 37 °C. Serum titres less than 1/2 (final dilution) are considered negative. If undiluted serum samples are toxic to the tissue cultures, these sera may be diluted 1/2 before being used in the test. This will be equivalent to 1/4 final dilution of serum. Serum titres of less than 1/4 (final dilution) are considered negative in these cases.

    Swine vesicular disease (SVD)

    Tests for swine vesicular disease (SVD) shall be carried out according to Commission Decision 2000/428/EC.

    Classical swine fever (CSF)

    Tests for classical swine fever (CSF) shall be carried out according to Commission Decision 2002/106/EC.

    The performance of tests for CSF should follow the guidelines set out in the OIE Manual of Standards for Diagnostic Tests and Vaccines — Chapter 2.1.13.

    The sensitivity and specificity of the serological test for CSF should be carried out by a national laboratory with a quality assurance scheme in place. Tests employed must be shown to recognise a range of weak and strong positive reference sera and allow detection of antibody in early phase and convalescence.




    ANNEX II (FRESH MEAT)

    PART 1

    List of third countries or parts thereof



    Country

    Code of territory

    Description of territory

    Veterinary certificate

    Specific conditions

    Model(s)

    SG

    1

    2

    3

    4

    5

    6

    AL — Albania

    AL-0

    Whole country

    -

     
     

    AR — Argentina

    AR-0

    Whole country

    EQU

     
     

    AR-1

    The provinces of Buenos Aires, Catamarca, Chaco, Corrientes, Entre Ríos, Formosa (except the territory of Ramon Lista), Jujuy, La Pampa, La Rioja, Mendoza, Misiones, Neuquen, Rio Negro, Salta (except the departments of General Jose de San Martin, Rivadavia, Oran, Iruya, and Santa Victoria), San Juan, San Luis, Santa Fe, Santiago del Estero, and Tucuman.

    BOV

    A

    1 and 2

    AR-2

    La Pampa and Santiago del Estero

    BOV

    A

    1 and 2

    AR-3

    Cordoba

    BOV

    A

    1 and 2

    AR-4

    Chubut, Santa Cruz and Tierra del Fuego

    BOV, OVI

     
     

    AR-5

    Formosa (only the territory of Ramon Lista) and Salta (only the department of Rivadavia)

    BOV

    A

    1 and 2

    AR-6

    Salta (only the departments of General Jose de San Martin, Oran, Iruya, and Santa Victoria)

    BOV

    A

    1 and 2

    AU — Australia

    AU-0

    Whole country

    BOV, OVI, POR, EQU, RUF, RUW, SUF, SUW

     
     

    BA — Bosnia and Herzegovina

    BA-0

    Whole country

    -

     
     

    BG — Bulgaria

    BG-0

    Whole country

    EQU

     
     

    BG-1

    The provinces of Varna, Dobrich, Silistra, Choumen, Targovitchte, Razgrad, Rousse, V.Tarnovo, Gabrovo, Pleven, Lovetch, Plovdic, Smolian, Pasardjik, Sofia district, Sofia city, Pernik, Kustendil, Blagoevgrad, Vratza, Montana and Vidin

    BOV, OVI, RUW, RUF

     
     

    BG-2

    The provinces of Bourgas, Jambol, Sliven, Starazagora, Hasskovo and Kardjali, excluding the 20 km wide corridor on the border with Turkey

     
     
     

    BH — Bahrain

    BH-0

    Whole country

    -

     
     

    BR — Brazil

    BR-0

    Whole country

    EQU

     
     

    BR-1

    States of Paraná, Minas Gerais (except regional delegations of Oliveira, Passos, São Gonçalo de Sapucai, Setelagoas and Bambuí), São Paulo, Espíritu Santo, Mato Grosso do Sul (except for the municipalities of Sete Quedas, Sonora, Aquidauana, Bodoqueno, Bonito, Caracol, Coxim, Jardim, Ladario, Miranda, Pedro Gomes, Porto Murtinho, Rio Negro, Rio Verde of Mato Grosso and Corumbá), Santa Catarina, Goias and the regional units of Cuiaba (except for the municipalities of San Antonio de Leverger, Nossa Senhora do Livramento, Pocone and Barão de Melgaço), Caceres (except for the municipality of Caceres), Lucas do Rio Verde, Rondonopolis (except for the municipality of Itiquiora), Barra do Garça and Barra do Burges in Mato Grosso.

    BOV

    A

    1 and 2

    BR-2

    State of Rio Grande do Sul

    BOV

    A

    1 and 2

    BR-3

    State of Mato Grosso do Sul, municipality of Sete Quedas

    BOV

    A

    1 and 2

    BW — Botswana

    BW-0

    Whole country

    EQU, EQW

     
     

    BW-1

    The veterinary disease control zones 5, 6, 7, 8, 9 and 18

    BOV, OVI, RUF, RUW

    F

    1 and 2

    BW-2

    The veterinary disease control zones 10, 11, 12, 13 and 14

    BOV, OVI, RUF, RUW

    F

    1 and 2

    BY — Belarus

    BY-0

    Whole country

    -

     
     

    BZ — Belize

    BZ-0

    Whole country

    BOV, EQU

     
     

    CA — Canada

    CA-0

    Whole country

    BOV, OVI, POR, EQU, SUF, SUW

    RUF, RUW,

     
     

    CH — Switzerland

    CH-0

    Whole country

    BOV, OVI, POR, EQU, RUF, RUW, SUF, SUW

     
     

    CL — Chile

    CL-0

    Whole country

    BOV, OVI, POR, EQU, RUF, RUW

     
     

    CN — China (People's Republic of)

    CN-0

    Whole country

    -

     
     

    CO — Colombia

    CO-0

    Whole country

    EQU

     
     

    CO-1

    The zone included within the borderlines from the point where the Murri River flows into the Atrato River, downstream along the Atrato River to where it flows into the Atlantic Ocean from this point to the Panamanian border following the Atlantic coastline to Cabo Tiburón; from this point to the Pacific Ocean following the Columbian-Panamanian border; from this point to the mouth of the Valle River along the Pacific coast and from this point along a straight line to the point where the Murri River flows into the Atrato River.

    BOV

    A

    2

    CO-2

    The municipalities of Arboletas, Necocli, San Pedro de Urah, Turbo, Apartado, Chigorodo, Mutata, Daheiba, Uramita, Murindo, Riosucio (right bank of the Atrato river) and Frontino.

    EQU

     
     

    CO-3

    The zone included within the borderlines from the mouth of the Sinu River on the Atlantic Ocean, upstream along the Sinu River to its head-Waters of Alto Paramillo, from this point to Puerto Rey on the Atlantic Ocean, following the borderline between the Department of Antiquia and Córdoba, and from this point to the mouth of the Sinu River along the Atlantic coast.

    BOV

    A

    2

    CR — Costa Rica

    CR-0

    Whole country

    BOV, EQU

     
     

    CU — Cuba

    CU-0

    Whole country

    BOV, EQU

     
     

    CY — Cyprus

    CY-0

    Whole country

    BOV, OVI, POR, EQU, RUF, RUW, SUF, SUW

     
     

    CZ — Czech Republic

    CZ-0

    Whole country

    BOV, OVI, EQU, RUW, RUF, POR, SUF

     
     

    CZ-1

    Whole country, except the provinces of Kromeriz, Vyskov, Hodonin, Uherske, Hradiste, Zlin and Vsetin

    SUW

     
     

    DZ — Algeria

    DZ-0

    Whole country

    -

     
     

    EE — Estonia

    EE-0

    Whole country

    RUW, RUF

     
     

    POR

    D

     

    ET — Ethiopia

    ET-0

    Whole country

    -

     
     

    FK — Falkland Islands

    FK-0

    Whole country

    BOV, OVI, EQU

     
     

    GL — Greenland

    GL-0

    Whole country

    BOV, OVI, EQU, RUF, RUW

     
     

    GT — Guatemala

    GT-0

    Whole country

    BOV, EQU

     
     

    HK — Hong Kong

    HK-0

    Whole country

    -

     
     

    HN — Honduras

    HN-0

    Whole country

    BOV, EQU

     
     

    HR — Croatia

    HR-0

    Whole country

    BOV, OVI, EQU, RUF, RUW

     
     

    HU — Hungary

    HU-0

    Whole country

    BOV, POR, OVI, EQU, RUW, RUF, SUF

     
     

    SUW

    C

     

    IL — Israel

    IL-0

    Whole country

    -

     
     

    IN — India

    IN-0

    Whole country

    -

     
     

    IS — Iceland

    IS-0

    Whole country

    BOV, OVI, EQU

     
     

    KE — Kenya

    KE-0

    Whole country

    -

     
     

    LT — Lithuania

    LT-0

    Whole country

    BOV, OVI, EQU, RUW, RUF

     
     

    POR

    D

     

    LV — Latvia

    LV-0

    Whole country

    RUW, RUF

     
     

    MA — Morocco

    MA-0

    Whole country

    EQU

     
     

    MG — Madagascar

    MG-0

    Whole country

    -

     
     

    MK — Former Yugoslav Republic of Macedonia (1)

    MK-0

    Whole country

    OVI, EQU

     
     

    MT — Malta

    MT-0

    Whole country

    BOV, POR, EQU

     
     

    MU — Mauritius

    MU-0

    Whole country

    -

     
     

    MX — Mexico

    MX-0

    Whole country

    BOV, EQU

     
     

    NA — Namibia

    NA-0

    Whole country

    EQU, EQW

     
     

    NA-1

    South of the cordon fences which extend from Palgrave Point in the west to Gam in the east

    BOV, OVI, RUF, RUW

    F

    2

    NC — New Caledonia

    NC-0

    Whole country

    BOV, RUF, RUW

     
     

    NI — Nicaragua

    NI-0

    Whole country

    -

     
     

    NZ — New Zealand

    NZ-0

    Whole country

    In accordance with Commission Decision 2003/56/EC

     
     

    PA — Panamá

    PA-0

    Whole country

    BOV, EQU

     
     

    PL — Poland

    PL-0

    Whole country

    BOV, OVI, EQU, RUW, RUF

     
     

    POR

    D

     

    PY — Paraguay

    PY-0

    Whole country

    EQU

     
     

    PY-1

    Chaco central and San Pedro areas

    BOV

    A & F

    1 and 2

    RO — Romania

    RO-0

    Whole country

    BOV, OVI, EQU, RUW, RUF

     
     

    RU — Russian Federation

    RU-0

    Whole country

    -

     
     

    RU-1

    Region of Murmansk (Murmanskaya oblast)

    RUF

     
     

    SCG — Serbia and Montenegro

    SCG-0

    Whole country

    EQU

     
     

    SCG-1

    Whole country except the region of Kosovo and Metohija

    BOV, OVI

     
     

    SI — Slovenia

    SI-0

    Whole country

    BOV, OVI, EQU, RUW, RUF

     
     

    SK — Slovakia

    SK-0

    Whole country

     
     
     

    SK-1

    The District Veterinary and Food Administrations (DVFA) of Trnava (comprising Piešťany, Hlohovec and Trnava districts); Levice (comprising Levice district); Nitra (comprising Nitra and Zlaté Moravce districts); Topoľčany (comprising Topoľčany district); Nové Mesto nad Váhom (comprising Nové Mesto nad Váhom district); Trenčín (comprising Trenčín and Bánovce nad Bebravou districts) Prievidza (comprising Prievidza and Partizánske districts); Púchov (comprising Púchov and Ilava districts); Žiar nad Hronom (comprising Žiar nad Hronom, Žarnovica and Banská Štiavnica districts); Zvolen (comprising Zvolen and Detva districts); Banská Bystrica (comprising Banská Bystrica and Brezno districts).

    BOV, OVI, EQU, RUW, RUF

     
     

    SK-2

    The District Veterinary and Food Administrations (DVFA) of Bratislava mesto (comprising Bratislava I., II., III., IV. and V. districts); Senec (comprising Senec, Pezinok and Malacky districts); Dunajská Streda (comprising Dunajská Streda district); Galanta (comprising Galanta district); Senica (comprising Senica and Skalica districts); Nové Mesto nad Váhom (comprising Myjava district); Púchov (comprising Považská Bystrica district); Nové Zámky (comprising Nové Zámky district); Komárno (comprising Komárno district); Šaľa (comprising Šaľa district); Žilina (comprising Žilina and Bytča district); Dolný Kubín (comprising Dolný Kubín, Tvrdošín and Námestovo districts); Martin (comprising Martin and Turčianske Teplice districts); Liptovský Mikuláš (comprising Liptovský Mikuláš and Ružomberok districts); Lučenec (comprising Lučenec and Poltár districts); Veľký Krtíš (comprising Veľký Krtíš district); Rimavská Sobota (comprising Rimavská Sobota and Revúca districts); Zvolen (comprising Krupina district); Poprad (comprising Poprad, Kežmarok and Levoča districts); Prešov (comprising Prešov and Sabinov districts); Bardejov (comprising Bardejov district); Vranov nad Topľou (comprising Vranov nad Topľou district); Svidník (comprising Svidník and Stropkov districts); Humenné (comprising Humenné, Medzilaborce and Snina districts); Stará Ľubovňa (comprising Stará Ľubovňa district); Košice—mesto (comprising Košice I., II., III. and IV. districts); Košice—okolie (comprising Košice—okolie district); Michalovce (comprising Michalovce and Sobrance districts); Rožňava (comprising Rožňava district); Spišská Nová Ves (comprising Spišská Nová Ves and Gelnica districts) and Trebišov (comprising Trebišov district).

    BOV, OVI, EQU, RUW, RUF, POR

    D

     

    SV — El Salvador

    SV-0

    Whole country

    -

     
     

    SZ — Swaziland

    SZ-0

    Whole country

    EQU, EQW

     
     

    SZ-1

    Area west of the ‘red line’ fences which extends northwards from the river Usutu to the frontier with South Africa west of Nkalashane, but excluding the veterinary foot-and-mouth surveillance and vaccination control areas gazetted as a statutory instrument under legal notice No 51 of 2001

    BOV, RUF, RUW

    F

    2

    TH — Thailand

    TH-0

    Whole country

    -

     
     

    TN — Tunisia

    TN-0

    Whole country

    -

     
     

    TR — Turkey

    TR-0

    Whole country

    -

     
     

    TR-1

    The provinces of Amasya, Ankara, Aydin, Balikesir, Bursa, Cankiri, Corum, Denizli, Izmir, Kastamonu, Kutahya, Manisa, Usak, Yozgat and Kirikkale

    EQU

     
     

    UA — Ukraine

    UA-0

    Whole country

    -

     
     

    US — United States

    US-0

    Whole country

    BOV, OVI, POR, EQU, SUF, SUW, RUF, RUW

     
     

    UY — Uruguay

    UY-0

    Whole country

    EQU

     
     

    BOV

    A

    1

    OVI

    B

    1 and 2

    ZA — South Africa

    ZA-0

    Whole country

    EQU, EQW

     
     

    ZA-1

    The whole country except:

    — the part of the foot-and-mouth disease control area situated in the veterinary regions of Mpumalanga and Northern provinces, in the district of Ingwavuma of the veterinary region of Natal and in the border area with Botswana east of longitude 28°, and

    — the district of Camperdown, in the province of KwaZuluNatal

    BOV, OVI, RUF, RUW

    F

    2

    ZW — Zimbabwe

    ZW-0

    Whole country

    -

     
     

    (1)   Former Yugoslav Republic of Macedonia; provisional code that does not affect the definitive denomination of the country to be attributed after the conclusion of the negotiations currently taking place in the United Nations.

    (2)   No certificate laid down and fresh meat imports are not authorised.

    Specific conditions referred to in column 6

    ‘1’

    :

    Geographic and timing restrictions



    Code of Territory

    Veterinary certificate

    Time period/dates for which importation into the Community is authorised or not authorised in relation to dates of slaughter/killing of animals from which the meat was obtained

    Model

    SG

     
     

    AR-1

    BOV

    A

    Before and including 31 January 2002

    Not authorised

    After and including 1 February 2002

    Authorised

    AR-2

    BOV

    A

    Before and including 8 March 2002

    Not authorised

    After and including 9 March 2002

    Authorised

    AR-3

    BOV

    A

    Before and including 26 March 2002

    None

    After and including 27 March 2002

    Authorised

    AR-4

    BOV, OVI, RUM, RUF

    -

    Before and including 28 February 2002

    Not authorised

    After and including 1 March 2002

    Authorised

    AR-5

    BOV

    A

    Before and including 10 July 2003

    Authorised

    After and including 11 July 2003

    Not authorised

    AR-6

    BOV

    A

    Before and including 4 September 2003

    Authorised

    After and including 5 September 2003

    Not authorised

    BR-2

    BOV

    A

    Before and including 30 November 2001

    Not authorised

    After and including 1 December 2001

    Authorised

    BR-3

    BOV

    A

    Before and including 31 October 2002

    Authorised

    After and including 1 November 2002

    Not authorised

    BW-1

    BOV, OVI, RUM, RUF

    A

    Before and including 7 July 2002

    Not authorised

    After and including 8 July 2002 to 23 December 2002

    Authorised

    After and including 24 December 2002 to 6 June 2003

    Not authorised

    After and including 7 June 2003

    Authorised

    BW-2

    BOV, OVI, RUM, RUF

    A

    Before and including 6 March 2002

    Not authorised

    After and including 7 March 2002

    Authorised

    PY-1

    BOV

    A

    Before and including 31 August 2002

    Not authorised

    After and including 1 September 2002 to 19 February 2003

    Authorised

     
     
     

    After and including 20 February 2003

    Not authorised

    UY-0

    BOV, OVI

    A

    Before and including 31 October 2001

    Not authorised

    After and including 1 November 2001

    Authorised

    ‘2’

    :

    Category restrictions

    No offal authorised (except bovine diaphragm and masseter muscles).

    PART 2

    Models of veterinary certificates

    Model(s):

    ‘BOV’

    :

    Model of veterinary certificate for fresh meat of domestic bovine animals (Bos taurus, Bison bison, Bubalus bubalis and their cross-breeds)

    ‘POR’

    :

    Model of veterinary certificate for fresh meat of domestic porcine animals (Sus scrofa)

    ‘OVI’

    :

    Model of veterinary certificate for fresh meat of domestic sheep (Ovis aries) and goats (Capra hircus)

    ‘EQU’

    :

    Model of veterinary certificate for fresh meat of domestic equine animals (Equus caballus, Equus asinus and their cross-breeds)

    ‘RUF’

    :

    Model of veterinary certificate for fresh meat of farmed non-domestic animals other than suidae and solipeds

    ‘RUW’

    :

    Model of veterinary certificate for fresh meat of wild non-domestic animals other than suidae and solipeds

    ‘SUF’

    :

    Model of veterinary certificate for fresh meat of farmed non-domestic suidae

    ‘SUW’

    :

    Model of veterinary certificate for fresh meat of wild non-domestic suidae

    ‘EQW’

    :

    Model of veterinary certificate for fresh meat of wild non-domestic solipeds

    SG (Supplementary guarantees):

    ‘A’

    :

    guarantees regarding the maturation, pH measurement and deboning of fresh meat, excluding offal, certified according to the models of certificates BOV (point 10.6), OVI (point 10.6), RUF (point 10.7) and RUW (point 10.4)

    ‘B’

    :

    guarantees regarding matured trimmed offal as described in the model of certificate BOV (point 10.6)

    ‘C’

    :

    guarantees regarding laboratory test for classical swine fever in the carcases from which fresh meat certified according to the model of certificate SUW (point 10.3 a) was obtained

    ‘D’

    :

    guarantees regarding swill feed on holding(s) of animals from which fresh meat certified according to models of certificate POR (point 10.3 (d)) was obtained

    ‘E’

    :

    guarantees regarding tuberculosis test in the animals from where fresh meat certified according to the model of certificate BOV (point 10.4 (d)) was obtained

    ‘F’

    :

    guarantees regarding the maturation and deboning of fresh meat, excluding offal, certified according to the models of certificates BOV (point 10.6), OVI (point 10.6), RUF (point 10.7) and RUW (point 10.4)

    Notes

    (a) Veterinary certificates shall be produced by the exporting country, based on the models appearing in Part 2 of Annex II, according to the layout of the model that corresponds to the meats concerned. They shall contain, in the numbered order that appears in the model, the attestations that are required for any third country and, as the case may be, those supplementary guarantees that are required for the exporting third country or part thereof.

    (b) A separate and unique certificate must be provided for meat that is exported from a single territory appearing in columns 2 and 3 of Part 1 of Annex II which is consigned to the same destination and transported in the same railway wagon, lorry, aircraft or ship.

    (c) The original of each certificate shall consist of a single page, both sides, or, where more text is required, it shall be in such a form that all pages needed are part of an integrated whole and indivisible.

    (d) It shall be drawn up in at least one of the official languages of the EU Member State in which the inspection at the border post shall be carried out and of the EU Member State of destination. However, these Member States may allow other languages, if necessary, accompanied by an official translation.

    (e) If for reasons of identification of the items of the consignment (schedule in point 8.3 of the model of certificate), additional pages are attached to the certificate, these pages shall also be considered as forming part of the original of the certificate by the application of the signature and stamp of the certifying official veterinarian, in each of the pages.

    (f) When the certificate, including additional schedules referred to in (e), comprises more than one page, each page shall be numbered — (page number) of (total number of pages) — at the bottom and shall bear the code number of the certificate that has been designated by the competent authority at the top.

    (g) The original of the certificate must be completed and signed by an official veterinarian. In doing so, the competent authorities of the exporting country shall ensure that the principles of certification equivalent to those laid down in Council Directive 96/93/EC are followed.

    The colour of the signature shall be different to that of the printing. The same rule applies to stamps other than those embossed or watermarked.

    (h) The original of the certificate must accompany the consignment at the EU border inspection post.

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    ▼M55




    ANNEX IV



    List of the specifically designated border inspection posts referred to in Article 12b

    ISO code

    Member State

    BIP

    LT

    Lithuania

    As laid down in Decision 2001/881/EC for Lithuania

    LV

    Latvia

    As laid down in Decision 2001/881/EC for Latvia

    PL

    Poland

    As laid down in Decision 2001/881/EC for Poland



    ( 1 ) OJ No L 302, 31. 12. 1972, p. 28.

    ( 2 ) OJ No L 26, 31. 1. 1977, p. 81.

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