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变形链球菌葡糖基转移酶B蔗糖结合位点肽-霍乱毒素B亚基嵌合蛋白的免疫学特性

Immunologic characteristics of a Streptococcus mutans glucosyltransferase B sucrose-binding site peptide-cholera toxin B-subunit chimeric protein.

作者信息

Laloi P, Munro C L, Jones K R, Macrina F L

机构信息

Centre de Génetique Moléculaire et Cellulaire, UMR CNRS 106, Université Claude Bernard, Villeurbanne, France.

出版信息

Infect Immun. 1996 Jan;64(1):28-36. doi: 10.1128/iai.64.1.28-36.1996.

Abstract

Glucosyltranferases (Gtfs) produced by the mutans streptococci are recognized as virulence factors in dental caries, and the inhibition of Gtfs by secretory immunoglobulin A is predicted to provide protection against this disease. The basis of such mucosal immunity is linked to the ability to reliably stimulate production of secretory immunoglobulin A against Gtfs. In this regard, we are exploring the immunogenicities of various Gtf peptides genetically fused to the B subunit of cholera toxin (CTB), a known mucosal adjuvant. In this work, we have created a gene fusion linking the GtfB active-site (AS) peptide DANFDSIRVDAVDNVDADLLQIA to the amino terminus of CTB. This sequence, deduced from the nucleotide sequence of gtfB from Streptococcus mutans GS5, has been found to be strongly conserved in Gtfs from several mutans streptococci. We have purified this recombinant protein (AS:CTB) from Escherichia coli carrying the fusion gene under the control of the lactose operon promoter. This protein was immunogenic in rabbits and produced specific serum antibodies against both the Gtf peptide and the CTB moiety. The antiserum was tested for its ability to inhibit GtfB activity obtained from a mutant of S. mutans able to make only this enzyme and none of the other usual Gtfs or fructosyltransferase. Approximately 50% of the GtfB activity was inhibited in such assays. These results suggest that the AS of this enzyme is accessible to antibody binding and that this region of the protein may be considered a vulnerable target for vaccine design and development. The AS:CTB was able to bind GM1, ganglioside in enzyme-linked immunosorbent assays, indicating that the recombinant protein retained this property, which is though to be critical to the mucosal immunoadjuvant properties of CTB. Thus, this protein may be promising as a candidate anticaries vaccinogen alone or in combination with other Gtf peptides or conjugates.

摘要

变形链球菌产生的葡糖基转移酶(Gtfs)被认为是龋齿的致病因素,预计分泌型免疫球蛋白A对Gtfs的抑制作用可预防这种疾病。这种黏膜免疫的基础与可靠刺激针对Gtfs的分泌型免疫球蛋白A产生的能力有关。在这方面,我们正在探索与霍乱毒素(CTB)B亚基基因融合的各种Gtf肽的免疫原性,CTB是一种已知的黏膜佐剂。在这项工作中,我们构建了一个基因融合体,将GtfB活性位点(AS)肽DANFDSIRVDAVDNVDADLLQIA连接到CTB的氨基末端。该序列由变形链球菌GS5的gtfB核苷酸序列推导而来,已发现它在几种变形链球菌的Gtfs中高度保守。我们从携带在乳糖操纵子启动子控制下的融合基因的大肠杆菌中纯化了这种重组蛋白(AS:CTB)。这种蛋白在兔中具有免疫原性,并产生了针对Gtf肽和CTB部分的特异性血清抗体。测试了该抗血清抑制从仅能产生这种酶而不产生其他常见Gtfs或果糖基转移酶的变形链球菌突变体中获得的GtfB活性的能力。在这类试验中,约50%的GtfB活性受到抑制。这些结果表明该酶的活性位点可被抗体结合,并且该蛋白的这一区域可被视为疫苗设计和开发的易损靶点。在酶联免疫吸附试验中,AS:CTB能够结合神经节苷脂GM1,表明该重组蛋白保留了这一特性,而这一特性被认为对CTB的黏膜免疫佐剂特性至关重要。因此,这种蛋白单独或与其他Gtf肽或偶联物联合作为候选抗龋疫苗原可能很有前景。

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