首页> 美国卫生研究院文献>Infection and Immunity >Homology of the 70-kilodalton antigens from Mycobacterium leprae and Mycobacterium bovis with the Mycobacterium tuberculosis 71-kilodalton antigen and with the conserved heat shock protein 70 of eucaryotes.
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Homology of the 70-kilodalton antigens from Mycobacterium leprae and Mycobacterium bovis with the Mycobacterium tuberculosis 71-kilodalton antigen and with the conserved heat shock protein 70 of eucaryotes.

机译:来自麻风分枝杆菌和牛分枝杆菌的70-千达尔顿抗原与结核分枝杆菌71-千达尔顿抗原和真核生物的保守热激蛋白70的同源性。

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摘要

Two lambda gt11 recombinant clones, JKL2 and JKL15, each containing an insert coding for part of the highly immunogenic 70-kilodalton (kDa) protein antigen, were isolated from a Mycobacterium leprae genomic library by immunoscreening with the monoclonal antibody L7. Clone JKL2 contained the largest insert, 2.3 kilobase pairs. Nonoverlapping fragments of this insert were used as probes and showed strong hybridization to a number of Mycobacterium tuberculosis-lambda gt11 recombinants producing proteins recognized by an anti-M. tuberculosis 71-kDa monoclonal antibody, IT11. One clone from a recombinant Mycobacterium bovis library was also characterized by using L7, and the insert from this clone, B5bt, hybridized strongly to the M. leprae probes as well. The nucleotide sequence of the 1,037-base-pair coding region of the JKL2 M. leprae clone which encodes the carboxy-terminal half of the 70-kDa protein had extensive homology with genes from a number of species. In all cases, these genes, including the recently described Ag63 and Ag361 of Plasmodium falciparum, were found to be members of the heat shock protein 70 (hsp 70) family of genes. At the amino acid level, homology was maximal between amino acids 83 through 107 and 159 through 184, which showed extreme conservation (92 and 85% identity) with Escherichia coli DnaK amino acids 386 through 409 and 460 through 485, respectively, and was 51% homologous over the entire coding region (amino acids 1 through 344 of JKL2). In contrast, amino acids 129 through 158 had maximal homology with the phylogenetically more distant Xenopus laevis hsp70. Homology declined substantially in the carboxy-terminal 34 amino acids. The predicted ATP-binding functional activity of the 70-kDa antigen from M. bovis was confirmed with affinity purification of the antigen by binding to ATP-agarose and elution with ATP. In view of the conservation of sequences between these mycobacterial antigens and mammalian endogenous cellular enzymes, further evaluation of these molecules in vivo may aid in understanding tolerance to self-antigens as well as provide potentially useful immunodiagnostic reagents.
机译:通过用单克隆抗体L7进行免疫筛选,从麻风分枝杆菌基因组文库中分离出两个λgt11重组克隆JKL2和JKL15,每个克隆均包含编码部分高度免疫原性70-千达尔顿(kDa)蛋白抗原的插入片段。克隆JKL2包含最大的插入片段,为2.3碱基对。该插入物的非重叠片段用作探针,并显示出与许多结核分枝杆菌-λgt11重组体的强杂交,这些重组体可产生被抗-M识别的蛋白质。结核71-kDa单克隆抗体,IT11。还使用L7对重组牛分枝杆菌文库中的一个克隆进行了表征,并且该克隆的插入片段B5bt也与麻风分枝杆菌探针强烈杂交。 JKL2麻疯树克隆的1,037个碱基对的编码区的核苷酸序列,编码70 kDa蛋白的羧基末端一半,与来自许多物种的基因具有广泛的同源性。在所有情况下,这些基因,包括最近描述的恶性疟原虫的Ag63和Ag361,都是热休克蛋白70(hsp 70)家族的成员。在氨基酸水平上,氨基酸83至107和159至184之间的同源性最大,分别显示与大肠杆菌DnaK氨基酸386至409和460至485的极端保守性(92和85%的同一性),为51在整个编码区(JKL2的氨基酸1至344)同源的%。相反,第129至158位氨基酸与系统发育较远的非洲爪蟾hsp70具有最大同源性。羧基末端34个氨基酸的同源性显着下降。通过与ATP-琼脂糖结合并用ATP洗脱进行抗原亲和纯化,证实了来自牛分枝杆菌的70-kDa抗原的预期ATP结合功能活性。考虑到这些分枝杆菌抗原和哺乳动物内源性细胞酶之间的序列的保守性,在体内对这些分子的进一步评估可以帮助理解对自身抗原的耐受性并提供潜在有用的免疫诊断试剂。

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