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粗糙脉孢菌漆酶去阻遏突变体的分离与鉴定

Isolation and characterization of a laccase-derepressed mutant of Neurospora crassa.

作者信息

Tamaru H, Inoue H

机构信息

Department of Regulation Biology, Faculty of Science, Saitama University, Urawa, Japan.

出版信息

J Bacteriol. 1989 Nov;171(11):6288-93. doi: 10.1128/jb.171.11.6288-6293.1989.

Abstract

Laccase from the ascomycete Neurospora crassa is an inducible secretory enzyme. Production of this enzyme is repressed in vegetative cultures but can be induced by treatment with low concentrations of cycloheximide. Isolation and characterization of a derepressed mutant, the lah-1 mutant, that is capable of producing laccase in vegetative cultures without induction by cycloheximide are described. The lah-1 mutation is mapped between nit-2 and leu-3 on linkage group I, and it behaved as a recessive mutation in a forced heterokaryon. No differences were detected biochemically or immunologically between the laccase protein produced by the lah-1 mutant in the absence of cycloheximide and that induced with cycloheximide in the wild-type strain. This suggests that both laccases (66 kilodaltons) are products of the same structural gene. Relative amounts of laccase in the culture filtrate of the lah-1 mutant were much higher than those induced with cycloheximide in the wild-type strain, demonstrating high efficiency of the lah-1 mutant in production and secretion of laccase. The time course of laccase production by the lah-1 mutant revealed that expression of 66-kilodalton laccase was repressed in conidia and derepressed during vegetative mycelial growth. This suggests that a multiple regulatory mechanism is involved in the production and/or maturation of Neurospora laccase. The lah-1 mutant may be useful for identifying genes that regulate expression of the laccase gene in N. crassa.

摘要

来自子囊菌粗糙脉孢菌的漆酶是一种诱导型分泌酶。在营养培养物中这种酶的产生受到抑制,但用低浓度的环己酰亚胺处理可诱导其产生。本文描述了一种去阻遏突变体lah-1突变体的分离和特性,该突变体能够在营养培养物中产生漆酶而无需用环己酰亚胺诱导。lah-1突变位于连锁群I上的nit-2和leu-3之间,在强制异核体中表现为隐性突变。在没有环己酰亚胺的情况下lah-1突变体产生的漆酶蛋白与野生型菌株用环己酰亚胺诱导产生的漆酶蛋白在生化或免疫方面未检测到差异。这表明两种漆酶(66千道尔顿)是同一结构基因的产物。lah-1突变体培养滤液中漆酶的相对含量远高于野生型菌株用环己酰亚胺诱导产生的含量,表明lah-1突变体在漆酶的产生和分泌方面效率很高。lah-1突变体产生漆酶的时间进程表明,66千道尔顿漆酶的表达在分生孢子中受到抑制,在营养菌丝体生长过程中去阻遏。这表明一种多重调控机制参与了粗糙脉孢菌漆酶的产生和/或成熟。lah-1突变体可能有助于鉴定调控粗糙脉孢菌漆酶基因表达的基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f292/210501/63db59744fc5/jbacter00177-0540-a.jpg

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