PRODUCTION OF SALMONELLA SEROGROUP-D (O9)-SPECIFIC ENZYME-LINKED-IMMUNOSORBENT-ASSAY ANTIGEN

被引：0

作者：

KONRAD, H ^{[1
]}

SMITH, BP ^{[1
]}

DILLING, GW ^{[1
]}

HOUSE, JK ^{[1
]}

机构：

[1] UNIV CALIF DAVIS, SCH VET MED, DEPT MED & EPIDEMIOL, DAVIS, CA 95616 USA

来源：

AMERICAN JOURNAL OF VETERINARY RESEARCH | 1994年 / 55卷 / 12期

关键词：

D O I：

暂无

中图分类号：

S85 [动物医学（兽医学）];

学科分类号：

0906 ;

摘要：

Serologic testing to detect persistent IgG titer directed at Salmonella lipopolysaccharide (LPS) has proven useful in detecting Salmonella carrier cattle without clinical signs of disease and in seroepidemiologic studies. Although little cross-reactivity exists between most Salmonella serogroups, groups B (O1, 4 [5], 12) and D (O1, 9, 12) share somatic (LPS cell wall) antigens O1 and O12, which results in some cross-reactions. This may be unimportant in most instances, because group-B and group-D carriers need to be identified and culled. It may be desirable in some situations, such as when trying to control S dublin, to determine which serogroup is present in a given herd. For this reason, a procedure to produce a pure O9 group-D antigen was developed. Salmonella dublin (group D) was grown by use of standard procedures, and LPS was extracted by use of the phenol-water method. The LPS was then oxidized with sodium periodate, dialyzed, reduced with sodium borohydride, cleaved with hydrochloric acid, and again dialyzed. This procedure successfully cleaved the saccharides comprising O antigens 1 and 12, leaving a pure O9 ELISA antigen. Sera from cattle vaccinated or naturally infected with S typhimurium, S agona, and S schwarzengrund (all group B), S montevideo (group O1), and S dublin (group D) were tested by ELlSA using modified and unmodified antigens. When the ELISA antigen used was the chemically modified (pure O9) group-D antigen, elimination of cross-reactions confirmed the structural loss of crossreacting O1 and O12 antigens.

引用

页码：1647 / 1651

页数：5

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