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马链球菌兽疫亚种H46A染色体链激酶区域的基因组织

Genetic organization of the streptokinase region of the Streptococcus equisimilis H46A chromosome.

作者信息

Mechold U, Steiner K, Vettermann S, Malke H

机构信息

Institute for Molecular Biology, Jena University, Germany.

出版信息

Mol Gen Genet. 1993 Oct;241(1-2):129-40. doi: 10.1007/BF00280210.

DOI:10.1007/BF00280210
PMID:8232196
Abstract

The complete nucleotide sequences of four genes and one open reading frame (ORF1) adjacent to the streptokinase gene, skc, from Streptococcus equisimilis H46A were determined. These genes are encoded on the opposite DNA strand to skc and are arranged as follows: dexB-abc-lrp-skc-ORF1-rel. The dexB gene, coding for an alpha-glucosidase (M(r) 61,733), and abc, encoding an ABC transporter (M(r) 42,080), are similar to the dexB and msmK genes, respectively, from the multiple sugar metabolism operon of S. mutans. The lrp gene specifies a leucine-rich protein (M(r) 32,302) that has a leucine-zipper motif at its C-terminus. The function of the Lrp protein is not known but appeared to be detrimental when overexpressed in Escherichia coli. Although lrp appears not to be an essential gene, as judged by plasmid insertion mutagenesis, it is conserved in all streptococcal strains carrying a streptokinase gene. The rel gene showed significant homology to the E. coli relA and spoT genes involved in the stringent response to amino acid deprivation. Multiple alignment of the amino acid sequences of Rel (M(r) 83,913), RelA and SpoT revealed 59.4% homology of the primary structures. Northern hybridization analyses of the genes in the skc region showed skc to be transcribed most abundantly. In addition to transcripts for skc, monocistronic mRNAs were detected for all three genes divergently transcribed from skc. Although there was also some read-through transcription from lrp into abc, and from abc into dexB, the transcription pattern suggests a high degree of transcriptional and functional independence not only of skc but also abc and dexB. Prominent structural features in intergenic regions included a static DNA bending locus located upstream and a putative bidirectional transcription terminator downstream of skc.

摘要

测定了来自类马链球菌H46A的链激酶基因skc相邻的四个基因和一个开放阅读框(ORF1)的完整核苷酸序列。这些基因编码在与skc相反的DNA链上,排列如下:dexB-abc-lrp-skc-ORF1-rel。编码α-葡萄糖苷酶(分子量61,733)的dexB基因和编码ABC转运蛋白(分子量42,080)的abc基因,分别与变形链球菌多糖代谢操纵子中的dexB和msmK基因相似。lrp基因编码一种富含亮氨酸的蛋白质(分子量32,302),其C末端具有亮氨酸拉链基序。Lrp蛋白的功能尚不清楚,但在大肠杆菌中过表达时似乎具有有害作用。尽管通过质粒插入诱变判断lrp似乎不是必需基因,但在所有携带链激酶基因的链球菌菌株中它都是保守的。rel基因与参与对氨基酸饥饿的严紧反应的大肠杆菌relA和spoT基因显示出显著的同源性。Rel(分子量83,913)、RelA和SpoT氨基酸序列的多重比对显示一级结构的同源性为59.4%。对skc区域基因的Northern杂交分析表明skc转录最为丰富。除了skc的转录本外,还检测到从skc发散转录的所有三个基因的单顺反子mRNA。尽管也存在从lrp到abc以及从abc到dexB的一些通读转录,但转录模式表明不仅skc,而且abc和dexB都具有高度的转录和功能独立性。基因间区域的显著结构特征包括位于skc上游的一个静态DNA弯曲位点和下游的一个推定的双向转录终止子。

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