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GB/T 18646-2025: Diagnostic techniques for animal brucellosis
Status: Valid GB/T 18646: Evolution and historical versions
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Diagnostic techniques for animal brucellosis
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GB/T 18646-2025
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Diagnostic techniques for animal brucellosis
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PDF similar to GB/T 18646-2025
Basic data | Standard ID | GB/T 18646-2025 (GB/T18646-2025) | | Description (Translated English) | Diagnostic techniques for animal brucellosis | | Sector / Industry | National Standard (Recommended) | | Classification of Chinese Standard | B41 | | Classification of International Standard | 11.220 | | Word Count Estimation | 66,654 | | Date of Issue | 2025-05-30 | | Date of Implementation | 2025-12-01 | | Older Standard (superseded by this standard) | GB/T 18646-2018 | | Issuing agency(ies) | State Administration for Market Regulation, China National Standardization Administration | GB/T 18646-2025: Diagnostic techniques for animal brucellosis---This is a DRAFT version for illustration, not a final translation. Full copy of true-PDF in English version (including equations, symbols, images, flow-chart, tables, and figures etc.) will be manually/carefully translated upon your order.
National Standard of the People's Republic of China
ICS 11.220CCS B 41
Diagnostic technology of animal brucellosis
2025-05-30 Release
2025-12-01 Implementation
State Administration for Market Regulation
The National Standardization Administration issued
Replaces GB/T 18646-2018
Table of contents
Preface...Ⅴ
Introduction VI
1 Scope...1
2 Normative references ...1
3 Terms and Definitions 1
4 Abbreviations 1
5 Clinical diagnosis 2
5.1 Popular characteristics 2
5.2 Clinical symptoms 2
5.3 Pathological changes 3
5.4 Result determination 3
6 Sample collection, storage, transportation and processing ...3
6.1 Instruments and Equipment 3
6.2 Reagents and Materials 3
6.3 Sample collection 3
6.4 Sample transportation and storage 4
6.5 Sample processing 4
7 Etiological diagnosis methods 5
7.1 Modified Ziehl⁃Neelsen acid-fast staining...5
7.2 Isolation and identification of Brucella 6
7.3 Real-time fluorescence PCR method 7
7.4 Fluorescence RAA method 9
7.5 Multiplex PCR method...11
8 Immunological diagnostic methods...12
8.1 Standard serum 12
8.2 Red tiger plate agglutination test (RBT) 13
8.3 Tube Agglutination Test (SAT) 14
8.4 Complement fixation test (CFT) 17
8.5 Indirect ELISA antibody detection method (iELISA) ...22
8.6 Competitive ELISA Antibody Detection Method (cELISA) ...24
8.7 Fluorescence Polarization Assay (FPA) 26
8.8 Milk Ring Test (MRT) (for cattle only) 29
8.9 Immunochromatography Assay (ICA) ...30
9 Comprehensive judgment 30
9.1 Determination of animals suspected of Brucella infection 30
9.2 Determination of Brucella Infection in Animals 31
Appendix A (Informative) Applicability of the test method 32
Appendix B (Normative) Preparation of Brucella Culture Medium 33
B.1 Basic culture medium 33
B.2 Serum Glucose Medium 33
B.3 Selection medium 33
Appendix C (Normative) Preparation of Biochemical Reagents 34
C.1 Preparation of Crystal Violet Stock and Working Solutions 34
C.2 Preparation of oxidase test reagents 34
C.3 Urease activity test medium formula and preparation ...34
Appendix D (Normative) Biochemical Identification of Brucella Species and Biotypes 35
Appendix E (Normative) Primer and probe sequences for real-time fluorescence PCR, RAA and multiplex PCR ...37
Appendix F (Normative) Multiplex PCR Solution Preparation and Result Determination 39
F.1 TAE electrophoresis buffer 39
F.2 1.5% agarose gel...39
F.3 Multiplex PCR judgment criteria 39
Appendix G (Normative) Preparation of tube agglutination test (SAT) reagents 40
G.1 Physiological saline containing 0.5% phenol...40
G.2 10% sodium chloride solution containing 0.5% phenol...40
G.3 Preparation of reference turbidimetric tubes 40
Appendix H (Normative) Preparation and titer determination of complement fixation test (CFT) reagents 41
H.1 Preparation of dilution solution 41
H.2 Preparation of Sheep Red Blood Cell Suspension (2.5%) 41
H.3 Hemolysin titer determination 41
H.4 Complement preparation and titer determination 44
H.5 Determination of antigen titer...49
H.6 Preparation of hemolysis standard colorimetric tubes and determination of complement fixation test results ...50
H.7 Dilution and inactivation of serum to be tested 51
Appendix I (Normative) Preparation of ELISA Reagents ...52
I.1 Extraction of coated antigen LPS 52
I.2 Coating solution (0.05 mol/L pH 9.6 carbonate buffer) ...52
I.3 Blocking solution (PBS with 2% BSA and 0.05% Tween-20, pH 7.4) ...52
I.4 Sample diluent (PBS with 1% BSA, pH 7.4) ...52
I.5 Washing solution (PBS with 0.05% Tween-20, pH 7.4) ...52
I.6 Color developing solution 52
I.7 Stop solution (2 mol/L sulfuric acid) 53
Appendix J (Informative) Preparation of Monoclonal Antibodies for Competitive Enzyme-Linked Immunosorbent Assay (cELISA) 54
Appendix K (Normative) Preparation of Fluorescence Polarization Assay (FPA) Antigens and Dilutions 55
K.1 Preparation of labeled antigens 55
K.2 Preparation of sample diluent 55
References ...56
Foreword
This document is in accordance with the provisions of GB/T 1.1-2020 "Guidelines for standardization work Part 1.Structure and drafting rules for standardization documents"
Drafting is required.
This document replaces GB/T 18646-2018 "Diagnostic techniques for animal brucellosis". Compared with GB/T 18646-2018, except for the structure
In addition to adjustments and editorial changes, the main technical changes are as follows.
a) The “Scope” has been changed (see Chapter 1, Chapter 1 of the.2018 edition);
b) Changed “Clinical Diagnosis” and added content on epidemiology, clinical symptoms and pathological changes (see Chapter 5, 4.1,.2018 edition).
4.2, 4.3);
c) Added “real-time fluorescence PCR method” and “fluorescence RAA method” (see 7.3 and 7.4);
d) Change “Brucella Bruce-Ladder detection method” to “Multiplex PCR method” (see 7.5, 4.13 of the.2018 version);
e) Added the standardization content of RBT, SAT, CFT, iELISA, cELISA and FPA methods in immunological diagnostic methods (see
Chapter 8);
f) Changed the “Red tiger plate agglutination test (RBT)” (see 8.2, 4.4 of the.2018 edition), “Indirect ELISA antibody detection method
(iELISA)” (see 8.5, 4.8 of the.2018 edition), “competitive ELISA antibody detection method (cELISA)” (see 8.6,.2018
4.9 of the.2011 edition);
g) Added “Fluorescence polarization assay (FPA)” and “Immunochromatographic assay (ICA)” (see 8.7 and 8.9).
This document was proposed by the Ministry of Agriculture and Rural Affairs of the People's Republic of China.
This document is under the jurisdiction of the National Technical Committee on Animal Health Standardization (SAC/TC 181).
This document was drafted by. China Animal Health and Epidemiology Center, China Veterinary Drug Administration, China Animal Disease Prevention and Control Center
Center, Harbin Veterinary Research Institute of Chinese Academy of Agricultural Sciences, Chinese Center for Disease Control and Prevention, Xinjiang Production and Construction Corps Animal Husbandry and Veterinary Work General Office
Liaoning Provincial Animal Disease Prevention and Control Center, Inner Mongolia Autonomous Region Animal Disease Prevention and Control Center, Shanghai Animal Disease Prevention and Control Center
Center, Henan Provincial Animal Disease Prevention and Control Center, Chongqing Municipal Animal Disease Prevention and Control Center, Zhejiang Provincial Animal Disease Prevention and Control Center,
Qingdao Animal Disease Prevention and Control Center.
The main drafters of this document are. Sun Shufang, Li Junping, Shao Weixing, Sun Mingjun, Jiang Hai, Nan Wenlong, Tian Lili, Fan Xiaoxu, Yan Xin, Sun Yu,
Hu Sen, Li Yan, Zhu Liangquan, Wang Jianlong, Yan Ruoqian, Zhang Cunrui, Li Yan, Gu Guibo, Zhao Hongjin, Dong Chunxia, Zhao Lingyan, Guo Yu, Sun Xiangxiang, Liu Mengda,
Zhang Haobo, Sun Shixiong, and Li Jiaqi.
The previous versions of this document and the documents it replaces are as follows.
--First published in.2002 as GB/T 18646-2002 and first revised in.2018;
--This is the second revision.
Introduction
Brucellosis is a zoonotic infectious disease caused by Brucella infecting animals and humans.
The Brucella species reported so far include 6 classical species, 5 newly identified species, and some atypical Brucella species of unidentified types.
Classical species include Brucella melitensis, Brucella abortus, and Brucella suis.
cella suis), Brucella ovis, Brucella canis, and Brucella sarcoma
Brucella neotomae; newly identified species include Brucella ceti, Brucella pinnipedia
lis), Brucella microti, Brucella inopinata (other animal hosts have not yet been identified), and
Brucella papionis; unidentified species include atypical Brucella isolated from rodents, foxes, and frogs.
This document mainly stipulates the three smooth Brucella species, namely, Brucella melitensis, Brucella bovis and Brucella suis, which have the greatest impact on animal husbandry.
The diagnostic and detection technology content related to animal brucellosis caused by Bacillus thuringiensis only involves the rough type in pathogen identification and PCR detection method.
Detection of Brucella epididymis of sheep and canine species.
Brucellosis is a serious threat to animal and human health worldwide.
The World Animal Health Organization (WOAH) has included brucellosis in the list of notifiable diseases, and the Ministry of Agriculture and Rural Affairs of my country has issued the "List of Class I, II and III Animal Diseases".
The List of Disease Species lists brucellosis as a Category II animal disease, and the National Health Commission lists brucellosis as a Category II animal disease.
Personnel engaged in sample collection, packaging and transportation, testing and diagnosis related to brucellosis diagnosis must undergo rigorous training.
Conduct experimental activities under the appropriate level of biosafety protection conditions.
This document refers to Chapter 3.1.4 Brucellosis (bovine, ovine and porcine species) of the WOAH Manual of Diagnostic Tests and Vaccines for Terrestrial Animals.
The diagnostic techniques and methods specified in the "Brucei Infection (2022 Edition)" include clinical diagnosis, etiological diagnosis methods (smear microscopy, isolation and identification)
determination, real-time fluorescence PCR method) and immunological diagnostic methods [red tiger plate agglutination test (RBT), tube agglutination test (SAT), complement binding
Combined test (CFT), indirect ELISA antibody detection method (iELISA), competitive ELISA antibody detection method (cELISA), fluorescence polarization
test (FPA) and whole breast ring test (MRT)]; and according to the development of my country's technology, the mature fluorescent RAA method and immunoassay were added
Chromatography (ICA).
The issuing organization of this document calls attention to the fact that when declaring that the relevant product complies with this document, it may involve the primer and probe sequences in 7.3 of this document.
Listed together with "A Molecular Marker for Distinguishing Brucella A19 Vaccine Strain from Wild Strains" (Authorization Announcement No.. CN113186312B), "Identification of Brucella
The use of the related patent "SNP Molecular Markers of Bacillus Vaccine S2 and Wild Strains and Their Applications" (Authorization Announcement No.. CN111793704B).
The issuing organization of this document takes no position on the authenticity, validity and scope of the patents involved.
The patent holder has promised to the publisher of this document that it agrees to license the patent to any organization free of charge on a fair, reasonable and non-discriminatory basis.
Or an individual implements a patent when implementing the national standard. The statement of the patent holder has been filed with the issuing agency of this document. Related information
It can be obtained through the following contact information.
Patent (Grant Announcement No.. CN113186312B) Holder Name. China Animal Health and Epidemiology Center.
Address. No. 369, Nanjing Road, Shibei District, Qingdao City, Shandong Province.
Patent (Grant Announcement No.. CN111793704B) Holder Name. Institute of Communicable Disease Prevention and Control, Chinese Center for Disease Control and Prevention.
Address. No. 155, Changbai Road, Changping District, Beijing.
Please note that in addition to the above two patents, some of the contents of this document may still involve patents. The issuing agency of this document does not assume the responsibility for identifying
Patent liability.
Diagnostic technology of animal brucellosis
1 Scope
This document describes the clinical, etiological and immunological diagnostic methods for animal brucellosis and provides a comprehensive
Meet the judgment requirements.
This document is applicable to the monitoring of the freedom of herds and individual animals for brucellosis, implementation of eradication programmes, confirmation of suspected or clinical cases, and
diagnosis, population prevalence monitoring, etc.
Note. Appendix A lists in detail the selection of detection methods in different fields.
2 Normative references
The contents of the following documents constitute the essential clauses of this document through normative references in this document.
For referenced documents without a date, only the version corresponding to that date applies to this document; for referenced documents without a date, the latest version (including all amendments) applies to
This document.
NY/T 541 Technical Specification for Collection, Storage and Transportation of Veterinary Diagnostic Samples
3 Terms and definitions
There are no terms or definitions that require definition in this document.
4 Abbreviations
The following abbreviations apply to this document.
cELISA. Competitive Enzyme Linked Immunosorbent Assay
CFT. Complement Fixation Test
Ct. Cycle Threshold
DNA. Deoxyribonucleic Acid
FPA. Fluorescence Polarisation Assay
HRP. Horseradish Peroxidase
iELISA. Indirect Enzyme Linked Immunosorbent Assay
LPS. Lipopolysaccharide
OD value. Optical Density
PCR. Polymerase Chain Reaction
RAA. Recombinase Aided Amplification
RBT. Rose Bengal Test
SAT. Serum Agglutination Test
SDS. Sodium dodecyl sulfate
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