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一种新型外膜阴离子通道(孔蛋白),它是睾丸酮丛毛单胞菌T-2中4-甲苯磺酸盐推测性双组分转运系统的一部分。

A novel outer-membrane anion channel (porin) as part of a putatively two-component transport system for 4-toluenesulphonate in Comamonas testosteroni T-2.

作者信息

Mampel Jörg, Maier Elke, Tralau Tewes, Ruff Jürgen, Benz Roland, Cook Alasdair M

机构信息

Department of Biology, The University, D-78457 Konstanz, Germany.

出版信息

Biochem J. 2004 Oct 1;383(Pt 1):91-9. doi: 10.1042/BJ20040652.

Abstract

Inducible mineralization of TSA (4-toluenesulphonate) by Comamonas testosteroni T-2 is initiated by a secondary transport system, followed by oxygenation and oxidation by TsaMBCD to 4-sulphobenzoate under the regulation of TsaR and TsaQ. Evidence is presented for a novel, presumably two-component transport system (TsaST). It is proposed that TsaT, an outer-membrane porin, formed an anion-selective channel that works in co-operation with the putative secondary transporter, TsaS, located in the inner membrane. tsaT was identified as a 1017-bp ORF (open reading frame) on plasmid pTSA upstream of the TSA-catabolic genes in the tsa operon. Expression of tsaT was regulated by TsaR, the transcriptional activator of the tsa regulon. The presence of tsaT was concomitant with the presence of the tsa operon in different TSA-degrading isolates. tsaT was expressed in Escherichia coli and was detected in the outer membrane. A 22-amino-acid leader peptide was identified. Purified protein reconstituted in lipid bilayer membranes formed anion-selective channels with a single-channel conductance of 3.5 nS in 1 M KCl. Downstream of tsaT, a constitutively expressed 720-bp ORF (tsaS) was identified. tsaS coded for a hydrophobic protein predicted to have six transmembrane helices and which is most likely localized in the cytoplasmic membrane. tsaS is adjacent to tsaT, but showed a different transcriptional profile.

摘要

睾丸酮丛毛单胞菌T-2对对甲苯磺酸盐(TSA)的诱导矿化作用由一个次级转运系统启动,随后在TsaR和TsaQ的调控下,经TsaMBCD氧化为4-磺基苯甲酸。文中提供了一种新型的、可能是双组分转运系统(TsaST)的证据。有人提出,外膜孔蛋白TsaT形成了一个阴离子选择性通道,该通道与位于内膜的假定次级转运蛋白TsaS协同工作。tsaT被鉴定为位于tsa操纵子中TSA分解代谢基因上游的质粒pTSA上的一个1017 bp的开放阅读框(ORF)。tsaT的表达受tsa调控子的转录激活因子TsaR的调节。在不同的TSA降解菌株中,tsaT的存在与tsa操纵子的存在相伴。tsaT在大肠杆菌中表达,并在外膜中被检测到。鉴定出一个22个氨基酸的前导肽。在脂质双分子层膜中重构的纯化蛋白形成了阴离子选择性通道,在1 M KCl中的单通道电导为3.5 nS。在tsaT的下游,鉴定出一个组成型表达的720 bp的开放阅读框(tsaS)。tsaS编码一种预测有六个跨膜螺旋的疏水蛋白,最有可能定位于细胞质膜。tsaS与tsaT相邻,但显示出不同的转录谱。

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