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嗜热栖热放线菌中支架蛋白相关基因表达的调控

Regulation of expression of scaffoldin-related genes in Clostridium thermocellum.

作者信息

Dror Tali W, Rolider Adi, Bayer Edward A, Lamed Raphael, Shoham Yuval

机构信息

Department of Food Engineering and Biotechnology, Technion-Israel Institute of Technology, Haifa, Israel.

出版信息

J Bacteriol. 2003 Sep;185(17):5109-16. doi: 10.1128/JB.185.17.5109-5116.2003.

DOI:10.1128/JB.185.17.5109-5116.2003
PMID:12923083
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC181014/
Abstract

Clostridium thermocellum produces an extracellular multienzyme complex, termed the cellulosome, that allows efficient solubilization of crystalline cellulose. The complex is organized around a large noncatalytic protein subunit, termed CipA or scaffoldin, and is found either free in the supernatant or cell bound. The binding of the complex to the cell is mediated by three cell surface anchoring proteins, OlpB, Orf2p, and SdbA, that interact with the CipA scaffoldin. The transcriptional level of the olpB, orf2, sdbA, and cipA genes was determined quantitatively by RNase protection assays in batch and continuous cultures, under carbon and nitrogen limitation. The mRNA level of olpB, orf2, and cipA varied with growth rate, reaching 40 to 60 transcripts per cell under carbon limitation at a low growth rate of 0.04 h(-1) and 2 to 10 transcripts per cell at a growth rate of 0.35 h(-1) in batch culture. The mRNA level of sdbA was about three transcripts per cell and was not influenced by growth rate. Primer extension analysis revealed two major transcriptional start sites, at -81 and -50 bp, upstream of the translational start site of the cipA gene. The potential promoters exhibited homology to the known sigma factors sigma(A) and sigma(L) (sigma(54)) of Bacillus subtilis. Transcription from the sigma(L)-like promoter was found under all growth conditions, whereas transcription from the sigma(A)-like promoter was significant only under carbon limitation. The overall expression level obtained in the primer extension analysis was in good agreement with the results of the RNase-protection assays.

摘要

嗜热栖热菌产生一种细胞外多酶复合物,称为纤维小体,它能有效地溶解结晶纤维素。该复合物围绕着一个大的非催化蛋白亚基(称为CipA或支架蛋白)组装而成,可游离于上清液中,也可结合在细胞上。该复合物与细胞的结合由三种细胞表面锚定蛋白OlpB、Orf2p和SdbA介导,它们与CipA支架蛋白相互作用。在分批培养和连续培养中,在碳和氮限制条件下,通过核糖核酸酶保护试验定量测定olpB、orf2、sdbA和cipA基因的转录水平。olpB、orf2和cipA的mRNA水平随生长速率而变化,在分批培养中,碳限制条件下生长速率为0.04 h⁻¹时,每个细胞达到40至60个转录本,生长速率为0.35 h⁻¹时,每个细胞为2至10个转录本。sdbA的mRNA水平约为每个细胞三个转录本,不受生长速率影响。引物延伸分析揭示了cipA基因翻译起始位点上游-81和-50 bp处的两个主要转录起始位点。潜在启动子与枯草芽孢杆菌已知的σ因子σ(A)和σ(L)(σ(54))具有同源性。在所有生长条件下均发现来自σ(L)样启动子的转录,而来自σ(A)样启动子的转录仅在碳限制条件下显著。引物延伸分析中获得的总体表达水平与核糖核酸酶保护试验的结果高度一致。