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嗜热紫链霉菌OPC-520高亲和力木二糖转运蛋白的分子特征及其转录调控

Molecular characterization of a high-affinity xylobiose transporter of Streptomyces thermoviolaceus OPC-520 and its transcriptional regulation.

作者信息

Tsujibo Hiroshi, Kosaka Mitsuo, Ikenishi Sadao, Sato Takaji, Miyamoto Katsushiro, Inamori Yoshihiko

机构信息

Department of Microbiology, Osaka University of Pharmaceutical Sciences, Takatsuki, Osaka 569-1094, Japan.

出版信息

J Bacteriol. 2004 Feb;186(4):1029-37. doi: 10.1128/JB.186.4.1029-1037.2004.

Abstract

Streptomyces thermoviolaceus OPC-520 secretes two types of xylanases (StxI and StxII), an acetyl xylan esterase (StxIII), and an alpha-L-arabinofuranosidase (StxIV) in the presence of xylan. Xylan degradation products (mainly xylobiose) produced by the action of these enzymes entered the cell and were then degraded to xylose by an intracellular beta-xylosidase (BxlA). A gene cluster involved in xylanolytic system of the strain was cloned and sequenced upstream of and including a BxlA-encoding gene (bxlA). The gene cluster consisted of four different open reading frames organized in the order bxlE, bxlF, bxlG, and bxlA. Reverse transcriptase PCR analysis revealed that the gene cluster is transcribed as polycistronic mRNA. The deduced gene products, comprising BxlE (a sugar-binding lipoprotein), BxlF (an integral membrane protein), and BxlG (an integral membrane protein), showed similarity to components of the bacterial ATP-binding cassette (ABC) transport system; however, the gene for the ATP binding protein was not linked to the bxl operon. The soluble recombinant BxlE protein was analyzed for its binding activity for xylooligosaccharides. The protein showed high-level affinity for xylobiose (K(d) = 8.75 x 10(-9) M) and for xylotriose (K(d) = 8.42 x 10(-8) M). Antibodies raised against the recombinant BxlE recognized the detergent-soluble BxlE isolated from S. thermoviolaceus membranes. The deduced BxlF and BxlG proteins are predicted to be integral membrane proteins. These proteins contained the conserved EAA loop (between the fourth and the fifth membrane-spanning segments) which is characteristic of membrane proteins from binding-protein-dependent ABC transporters. In addition, the bxlR gene located upstream of the bxl operon was cloned and expressed in Escherichia coli. The bxlR gene encoded a 343-residue polypeptide that is highly homologous to members of the GalR/LacI family of bacterial transcriptional regulators. The purified BxlR protein specifically bound to a 4-bp inverted sequence overlapping the -10 region of the bxl operon. The binding of BxlR to the site was inhibited specifically by low concentrations of xylobiose. This site was also present in the region located between stxI and stxIV and in the upstream region of stxII. BxlR specifically bound to the regions containing the inverted sequence. These results suggest that BxlR might act as a repressor of the genes involved not only in the uptake system of xylan degradation products but also in xylan degradation of S. thermoviolaceus OPC-520.

摘要

嗜热紫链霉菌OPC-520在木聚糖存在的情况下会分泌两种木聚糖酶(StxI和StxII)、一种乙酰木聚糖酯酶(StxIII)和一种α-L-阿拉伯呋喃糖苷酶(StxIV)。这些酶作用产生的木聚糖降解产物(主要是木二糖)进入细胞,然后被细胞内的β-木糖苷酶(BxlA)降解为木糖。克隆并测序了该菌株木聚糖分解系统相关的基因簇,其位于编码BxlA的基因(bxlA)上游且包含该基因。该基因簇由四个不同的开放阅读框组成,排列顺序为bxlE、bxlF、bxlG和bxlA。逆转录酶PCR分析表明,该基因簇转录为多顺反子mRNA。推导的基因产物包括BxlE(一种糖结合脂蛋白)、BxlF(一种整合膜蛋白)和BxlG(一种整合膜蛋白),与细菌ATP结合盒(ABC)转运系统的组分相似;然而,ATP结合蛋白的基因未与bxl操纵子相连。分析了可溶性重组BxlE蛋白对木寡糖的结合活性。该蛋白对木二糖(K(d)=8.75×10(-9)M)和木三糖(K(d)=8.42×10(-8)M)表现出高亲和力。针对重组BxlE产生的抗体识别从嗜热紫链霉菌膜中分离出的去污剂可溶的BxlE。推导的BxlF和BxlG蛋白预计为整合膜蛋白。这些蛋白含有保守的EAA环(在第四和第五个跨膜区段之间),这是依赖结合蛋白的ABC转运体膜蛋白的特征。此外,克隆了位于bxl操纵子上游的bxlR基因并在大肠杆菌中表达。bxlR基因编码一个343个残基的多肽,与细菌转录调节因子GalR/LacI家族的成员高度同源。纯化的BxlR蛋白特异性结合与bxl操纵子-10区重叠的4个碱基的反向序列。低浓度的木二糖可特异性抑制BxlR与该位点的结合。该位点也存在于stxI和stxIV之间的区域以及stxII的上游区域。BxlR特异性结合含有反向序列的区域。这些结果表明,BxlR可能不仅作为参与木聚糖降解产物摄取系统的基因的阻遏物,而且作为嗜热紫链霉菌OPC-520木聚糖降解相关基因的阻遏物发挥作用。

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