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Cloning, nucleotide sequence, and mutagenesis of a gene (irpA) involved in iron-deficient growth of the cyanobacterium Synechococcus sp. strain PCC7942.

机译:克隆,核苷酸序列和诱变的基因(irpA)参与缺铁的蓝藻Syechococcus sp。菌株PCC7942。

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摘要

We describe the cloning and sequencing of a gene from the cyanobacterium Synechococcus sp. strain PCC7942, designated irpA (iron-regulated protein A), that encodes for a protein involved in iron acquisition or storage. Polyclonal antibodies raised against proteins which accumulate during iron-deficient growth were used as probes to isolate immunopositive clones from a lambda gt11 genomic expression library. The clone, designated lambda gtAN26, carried a 1.7-kilobase (kb) chromosomal DNA insert and was detected by cross-reactivity with antibody against a 36-kilodalton protein. It was possible to map a 20-kb portion of the chromosome with various DNA probes from lambda gt11 and lambda EMBL-3 clones, and Southern blot analysis revealed that the irpA gene was present in a single copy and localized within a 1.7-kb PstI fragment. DNA sequencing revealed an open reading frame of 1,068 nucleotides capable of encoding 356 amino acids which yields a protein with a molecular weight of 38,584. The hydropathy profile of the polypeptide indicated a putative N-terminal signal sequence of 44 amino acid residues. IrpA is a cytoplasmic membrane protein as determined by biochemistry and electron microscopy immunocytochemistry. The upstream region of the irpA gene contained a consensus sequence similar to the aerobactin operator in Escherichia coli. This fact, plus a mutant with a mutation in irpA that is unable to grow under iron-deficient conditions, led us to suggest that irpA is regulated by iron and that the gene product is involved in iron acquisition or storage.
机译:我们描述了从蓝细菌Synchococcus sp。克隆和测序的基因。菌株PCC7942,称为irpA(铁调节的蛋白A),编码与铁的获取或储存有关的蛋​​白。针对在铁缺乏的生长过程中积累的蛋白质产生的多克隆抗体被用作探针,以从λgt11基因组表达文库中分离出免疫阳性克隆。该克隆命名为λgtAN26,带有一个1.7碱基(kb)的染色体DNA插入片段,并通过与针对36公斤蛋白的抗体的交叉反应进行检测。可以用来自λgt11和λEMBL-3克隆的各种DNA探针定位染色体的20kb部分,Southern印迹分析表明irpA基因以单拷贝形式存在,并位于1.7kb PstI中分段。 DNA测序显示一个1,068个核苷酸的开放阅读框,能够编码356个氨基酸,从而产生分子量为38,584的蛋白质。多肽的亲水性谱表明推定的44个氨基酸残基的N-末端信号序列。通过生物化学和电子显微镜免疫细胞化学测定,IrpA是一种细胞质膜蛋白。 irpA基因的上游区域包含一个共有序列,类似于大肠杆菌中的航空细菌素操纵子。这个事实,加上在铁缺乏条件下无法生长的,具有irpA突变的突变体,使我们提出irpA受铁调节,并且基因产物参与铁的获取或储存。

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