Cloning and sequencing of a gene encoding acidophilic amylase from Bacillus acidocaldarius.

T T Koivula, H Hemilä, R Pakkanen, M Sibakov, I Palva
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引用次数: 30

Abstract

Two starch-degrading enzymes produced by Bacillus acidocaldarius (renamed as Alicyclobacillus acidocaldarius) were identified. According to SDS-PAGE, the apparent molecular masses of the enzymes were 90 and 160 kDa. Eight peptide fragments and the N-terminal end of the 90 kDa polypeptide were sequenced. An oligonucleotide, based on the amino acid sequence of a peptide fragment of the 90 kDa protein, was used to screen a lambda gt10 bank of B. acidocaldarius, and the region encoding the 90 kDa protein was cloned. Unexpectedly, the ORF continued upstream of the N terminus of the 90 kDa protein. The entire ORF was 1301 amino acids (aa) long (calculated molecular mass 140 kDa) and it was preceded by a putative ribosomal binding site and a promoter. Computer analysis showed that the 1301 aa protein was closely related to an alpha-amylase-pullulanase of Clostridium thermohydrosulfuricum. We suggest that the starch-degrading 160 kDa protein of B. acidocaldarius is an alpha-amylase-pullulanase, and the 90 kDa protein is a cleavage product of the 160 kDa protein. Another ORF, apparently in the same transcription unit, was found downstream from the amylase gene. It encoded a protein that was closely related to the maltose-binding protein of Escherichia coli.

嗜酸芽孢杆菌嗜酸淀粉酶基因的克隆与序列分析。
鉴定了酸芽孢杆菌(更名为酸芽孢杆菌)产生的两种淀粉降解酶。根据SDS-PAGE,酶的表观分子质量分别为90和160 kDa。测序了8个肽片段和90 kDa多肽的n端。基于90 kDa蛋白肽片段的氨基酸序列,利用寡核苷酸筛选了酸性藻的lambda gt10库,并克隆了编码90 kDa蛋白的区域。出乎意料的是,ORF继续在90 kDa蛋白的N端上游。整个ORF有1301个氨基酸(aa)长(计算分子质量为140 kDa),其前面有一个假定的核糖体结合位点和一个启动子。计算机分析表明,1301 aa蛋白与热硫氢梭菌的α -淀粉酶-普鲁兰酶密切相关。我们认为,酸枝双歧杆菌降解淀粉的160 kDa蛋白是α -淀粉酶-葡聚糖酶,而90 kDa蛋白是160 kDa蛋白的裂解产物。在淀粉酶基因的下游发现了另一个ORF,显然在相同的转录单元中。它编码了一种与大肠杆菌的麦芽糖结合蛋白密切相关的蛋白质。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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