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确定巴尔通体杆菌侵袭相关基因座B(IalB)蛋白在人类红细胞寄生中的直接作用。

Establishing a direct role for the Bartonella bacilliformis invasion-associated locus B (IalB) protein in human erythrocyte parasitism.

作者信息

Coleman S A, Minnick M F

机构信息

Division of Biological Sciences, The University of Montana, Missoula, Montana 59812, USA.

出版信息

Infect Immun. 2001 Jul;69(7):4373-81. doi: 10.1128/IAI.69.7.4373-4381.2001.

Abstract

The invasion-associated locus A and B genes (ialAB) of Bartonella bacilliformis were previously shown to confer an erythrocyte-invasive phenotype upon Escherichia coli, indirectly implicating their role in virulence. We report the first direct demonstration of a role for ialB as a virulence factor in B. bacilliformis. The presence of a secretory signal sequence and amino acid sequence similarity to two known outer membrane proteins involved in virulence suggested that IalB was an outer membrane protein. To develop an antiserum for protein localization, the ialB gene was cloned in frame into an expression vector with a six-histidine tag and under control of the lacZ promoter. The IalB fusion protein was purified by nickel affinity chromatography and used to raise polyclonal antibodies. IalB was initially localized to the bacterial membrane fraction. To further localize IalB, B. bacilliformis inner and outer membranes were fractionated by sucrose density gradient centrifugation and identified by appearance, buoyant density (rho), and cytochrome b content. Inner and outer membrane proteins were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), and IalB was positively identified by Western blot. Contrary to expectations, IalB was localized to the inner membrane of the pathogen. To directly demonstrate a role for IalB in erythrocyte parasitism, the B. bacilliformis ialB gene was disrupted by insertional mutagenesis. The resulting ialB mutant strain was complemented in trans with a replicative plasmid encoding the full-length ialB gene. PCR and high-stringency DNA hybridization confirmed mutagenesis and transcomplementation events. Abrogation and restoration of ialB expression was verified by SDS-PAGE and immunoblotting. In vitro virulence assays showed that mutagenesis of ialB decreased bacterial association and invasion of human erythrocytes by 47 to 53% relative to controls. Transcomplementation of ialB restored erythrocyte association and invasion rates to levels observed in the parental strain. These data provide direct evidence for IalB's role in erythrocyte parasitism and represent the first demonstration of molecular Koch's postulates for a Bartonella species.

摘要

先前已表明,杆状巴尔通体的侵袭相关基因座A和B基因(ialAB)可赋予大肠杆菌红细胞侵袭表型,这间接暗示了它们在毒力方面的作用。我们首次直接证明了ialB作为杆状巴尔通体毒力因子的作用。ialB存在分泌信号序列,且其氨基酸序列与两个已知的参与毒力的外膜蛋白相似,这表明IalB是一种外膜蛋白。为了制备用于蛋白质定位的抗血清,ialB基因被框内克隆到一个带有六个组氨酸标签且受lacZ启动子控制的表达载体中。IalB融合蛋白通过镍亲和层析纯化,并用于制备多克隆抗体。IalB最初定位于细菌膜组分。为了进一步定位IalB,通过蔗糖密度梯度离心对杆状巴尔通体的内膜和外膜进行分级分离,并通过外观、浮力密度(rho)和细胞色素b含量进行鉴定。通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳(SDS - PAGE)分析内膜和外膜蛋白,并通过蛋白质印迹法阳性鉴定IalB。与预期相反,IalB定位于病原体的内膜。为了直接证明IalB在红细胞寄生中的作用,通过插入诱变破坏杆状巴尔通体的ialB基因。所得的ialB突变株用编码全长ialB基因的复制质粒进行反式互补。PCR和高严谨度DNA杂交证实了诱变和反式互补事件。通过SDS - PAGE和免疫印迹验证了ialB表达的缺失和恢复。体外毒力试验表明,ialB诱变使细菌与人红细胞的结合和侵袭相对于对照降低了47%至53%。ialB的反式互补将红细胞结合和侵袭率恢复到亲本菌株中观察到的水平。这些数据为IalB在红细胞寄生中的作用提供了直接证据,并且代表了对巴尔通体属物种分子科赫法则的首次证明。

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