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梅毒螺旋体(苍白密螺旋体)加工后的富含亮氨酸重复序列蛋白TpLRR的分子特征及细胞定位

Molecular characterization and cellular localization of TpLRR, a processed leucine-rich repeat protein of Treponema pallidum, the syphilis spirochete.

作者信息

Shevchenko D V, Akins D R, Robinson E, Li M, Popova T G, Cox D L, Radolf J D

机构信息

Department of Internal Medicine, U.T. Southwestern Medical Center at Dallas, Texas 75235, USA.

出版信息

J Bacteriol. 1997 May;179(10):3188-95. doi: 10.1128/jb.179.10.3188-3195.1997.

Abstract

Automated Edman degradation was used to obtain N-terminal and internal amino acid sequences from a 26-kDa protein in isolated Treponema pallidum outer membranes (OMs). The resulting sequences enabled us to PCR amplify from T. pallidum DNA a 275-bp fragment of the corresponding gene. The complete nucleotide sequence of the gene was determined from fragments amplified by long-distance PCR. Primer extension verified the assigned translational start of the open reading frame (ORF) and putative upstream promoter elements. The ORF encoded a highly basic (pI 9.6) 26-kDa protein which contained an N-terminal 25-amino-acid leader peptide terminated by a signal peptidase I cleavage site. The mature protein contained seven tandemly spaced copies (as well as an eighth incomplete copy) of a leucine-rich repeat (LRR), a motif previously identified in a number of prokaryotic and eukaryotic proteins. Accordingly, the polypeptide was designated T. pallidum leucine-rich repeat protein (TpLRR). Although Triton X-114 phase partitioning showed that TpLRR was hydrophilic, cell localization studies showed that most of the antigen was associated with the peptidoglycan-cytoplasmic membrane complex rather than being freely soluble in the periplasmic space. Immunoblot studies showed that syphilis patients develop a weak antibody response to the antigen. Lastly, the lrr(T. pallidum) gene was mapped to a 60-kb SfiI-SpeI fragment of the T. pallidum chromosome which also contains the rrnA and flaA genes. The function(s) of TpLRR is currently unknown; however, protein-protein and/or protein-lipid interactions mediated by its LRR motifs may facilitate interactions between components of the T. pallidum cell envelope.

摘要

采用自动埃德曼降解法从分离出的梅毒螺旋体外膜(OMs)中的一种26 kDa蛋白质获取N端和内部氨基酸序列。所得序列使我们能够从梅毒螺旋体DNA中PCR扩增出相应基因的一个275 bp片段。通过长距离PCR扩增片段确定了该基因的完整核苷酸序列。引物延伸验证了开放阅读框(ORF)的指定翻译起始位点和假定的上游启动子元件。该ORF编码一种高度碱性(pI 9.6)的26 kDa蛋白质,其包含一个由信号肽酶I切割位点终止的N端25个氨基酸的前导肽。成熟蛋白包含富含亮氨酸重复序列(LRR)的七个串联重复拷贝(以及第八个不完整拷贝),该基序先前在许多原核和真核蛋白质中已被鉴定。因此,该多肽被命名为梅毒螺旋体富含亮氨酸重复蛋白(TpLRR)。尽管Triton X - 114相分配表明TpLRR是亲水性的,但细胞定位研究表明,大多数抗原与肽聚糖 - 细胞质膜复合物相关,而非自由溶解于周质空间。免疫印迹研究表明,梅毒患者对该抗原产生微弱的抗体反应。最后,lrr(梅毒螺旋体)基因被定位到梅毒螺旋体染色体的一个60 kb SfiI - SpeI片段上,该片段还包含rrnA和flaA基因。TpLRR的功能目前尚不清楚;然而,由其LRR基序介导的蛋白质 - 蛋白质和/或蛋白质 - 脂质相互作用可能促进梅毒螺旋体细胞包膜各成分之间的相互作用。

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