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肺炎链球菌转化所需的膜结合核酸酶EndA的遗传和结构特征

Genetic and structural characterization of endA. A membrane-bound nuclease required for transformation of Streptococcus pneumoniae.

作者信息

Puyet A, Greenberg B, Lacks S A

机构信息

Department of Biology, Brookhaven National Laboratory, Upton, NY 11973.

出版信息

J Mol Biol. 1990 Jun 20;213(4):727-38. doi: 10.1016/S0022-2836(05)80259-1.

Abstract

The endA gene encoding the membrane nuclease of Streptococcus pneumoniae, which is necessary for DNA uptake in genetic transformation, was cloned in a streptococcal vector. This was accomplished by insertional mutagenesis of the gene, cloning of the mutant allele, and substitution of the wild-type allele by chromosomal facilitation of plasmid establishment. Plasmids carrying the endA+ gene complemented cells with endA- in the chromosome to restore DNAase activity and transformability. Determination of its DNA sequence showed the gene to encode a 30 kDa protein, EndA, with a typical signal sequence for membrane transport at its amino end. In vitro synthesis of EndA showed the initial translation product to be enzymatically active without further processing. Comparison with EndA found in cell membranes indicated that the enzyme retained its signal sequence, which apparently anchored the otherwise hydrophilic protein to the membrane. From the nucleotide sequence in the vicinity of endA and the effect of various insertions and deletions, it appears that endA is the last gene in an operon containing at least two other genes. Neither of these upstream genes, nor the downstream gene, are essential for either cell viability or transformability.

摘要

编码肺炎链球菌膜核酸酶的endA基因在遗传转化中对DNA摄取是必需的,该基因被克隆到链球菌载体中。这是通过对该基因进行插入诱变、克隆突变等位基因以及通过促进质粒建立的染色体方法替换野生型等位基因来实现的。携带endA⁺基因的质粒补充了染色体中带有endA⁻的细胞,以恢复DNA酶活性和转化能力。对其DNA序列的测定表明该基因编码一种30 kDa的蛋白质EndA,其氨基末端具有典型的膜转运信号序列。EndA的体外合成表明初始翻译产物无需进一步加工即具有酶活性。与细胞膜中发现的EndA进行比较表明,该酶保留了其信号序列,该信号序列显然将原本亲水的蛋白质锚定在膜上。从endA附近的核苷酸序列以及各种插入和缺失的影响来看,endA似乎是一个操纵子中的最后一个基因,该操纵子至少还包含另外两个基因。这些上游基因和下游基因对细胞活力或转化能力都不是必需的。

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