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嗜糖栖热解纤维素菌celC假基因的β-甘露聚糖酶结构域的校正及其基因产物对硫酸盐浆的活性

Correction of the beta-mannanase domain of the celC pseudogene from Caldocellulosiruptor saccharolyticus and activity of the gene product on kraft pulp.

作者信息

Morris D D, Reeves R A, Gibbs M D, Saul D J, Bergquist P L

机构信息

Centre for Gene Technology, School of Biological Sciences, University of Auckland, New Zealand.

出版信息

Appl Environ Microbiol. 1995 Jun;61(6):2262-9. doi: 10.1128/aem.61.6.2262-2269.1995.

DOI:10.1128/aem.61.6.2262-2269.1995
PMID:7793947
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC167498/
Abstract

The celA, manA, and celB genes from Caldocellulosiruptor saccharolyticus compose a cellulase-hemicellulase gene cluster and are arranged on a 12-kb C. saccharolyticus genomic fragment of the recombinant lambda bacteriophage NZP lambda 2. The beginning of a fourth open reading frame (celC) which was homologous to the C. saccharolyticus manA and celA genes was located at the 3' end of the 12-kb NZP lambda 2 genomic fragment. Genome-walking PCR was used to isolate DNA fragments downstream of the C. saccharolyticus celB gene, and the entire nucleotide sequence of celC was obtained. From the preliminary nucleotide sequence, celC appeared to encode yet another multidomain bifunctional enzyme (CelC) consisting of an N-terminal endo-1,4-beta-D-glucanase domain (75% similar to CelA domain 1), two central cellulose-binding domains, and a C-terminal endo-1,4-beta-D-mannanase domain (98% similar to ManA domain 1). However, upon completion of the celC sequencing, two -1 frameshifts were identified in the region encoding the putative CelC mannanase domain. The isolated CelC mannanase domain exhibited no beta-mannanase activity, which supported this observation. Recombinant PCR was used to correct the celC frameshifts by inserting the appropriate nucleotides into the gene. The repaired celC fragment containing the base insertions (manB) expressed strong beta-mannanase activity on soluble mannan substrates and showed significant activity on kraft pulp as judged by the release of reducing sugars.

摘要

来自嗜糖栖热解纤维素菌(Caldocellulosiruptor saccharolyticus)的celA、manA和celB基因组成了一个纤维素酶-半纤维素酶基因簇,它们排列在重组λ噬菌体NZP λ2的一个12 kb嗜糖栖热解纤维素菌基因组片段上。与嗜糖栖热解纤维素菌manA和celA基因同源的第四个开放阅读框(celC)的起始位置位于12 kb NZP λ2基因组片段的3'端。采用基因组步移PCR技术分离嗜糖栖热解纤维素菌celB基因下游的DNA片段,获得了celC的完整核苷酸序列。从初步的核苷酸序列来看,celC似乎编码另一种多结构域双功能酶(CelC),该酶由一个N端内切-1,4-β-D-葡聚糖酶结构域(与CelA结构域1相似度为75%)、两个中央纤维素结合结构域和一个C端内切-1,4-β-D-甘露聚糖酶结构域(与ManA结构域1相似度为98%)组成。然而,在完成celC测序后,在编码假定的CelC甘露聚糖酶结构域的区域发现了两个-1移码突变。分离得到的CelC甘露聚糖酶结构域没有表现出β-甘露聚糖酶活性,这支持了这一观察结果。通过将适当的核苷酸插入基因中,采用重组PCR技术校正celC的移码突变。修复后的celC片段(含碱基插入,即manB)对可溶性甘露聚糖底物表现出很强的β-甘露聚糖酶活性,并且通过还原糖的释放量判断,其对硫酸盐浆也表现出显著活性。

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