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用参与嘧啶生物合成的同源基因(pyrG)对寄生曲霉进行转化。

Transformation of Aspergillus parasiticus with a homologous gene (pyrG) involved in pyrimidine biosynthesis.

作者信息

Skory C D, Horng J S, Pestka J J, Linz J E

机构信息

Department of Food Science and Human Nutrition, Michigan State University, East Lansing 48824.

出版信息

Appl Environ Microbiol. 1990 Nov;56(11):3315-20. doi: 10.1128/aem.56.11.3315-3320.1990.

DOI:10.1128/aem.56.11.3315-3320.1990
PMID:2176447
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC184948/
Abstract

The lack of efficient transformation methods for aflatoxigenic Aspergillus parasiticus has been a major constraint for the study of aflatoxin biosynthesis at the genetic level. A transformation system with efficiencies of 30 to 50 stable transformants per microgram of DNA was developed for A. parasiticus by using the homologous pyrG gene. The pyrG gene from A. parasiticus was isolated by in situ plaque hybridization of a lambda genomic DNA library. Uridine auxotrophs of A. parasiticus ATCC 36537, a mutant blocked in aflatoxin biosynthesis, were isolated by selection on 5-fluoroorotic acid following nitrosoguanidine mutagenesis. Isolates with mutations in the pyrG gene resulting in elimination of orotidine monophosphate (OMP) decarboxylase activity were detected by assaying cell extracts for their ability to convert [14C]OMP to [14C]UMP. Transformation of A. parasiticus pyrG protoplasts with the homologous pyrG gene restored the fungal cells to prototrophy. Enzymatic analysis of cell extracts of transformant clones demonstrated that these extracts had the ability to convert [14C]OMP to [14C]UMP. Southern analysis of DNA purified from transformant clones indicated that both pUC19 vector sequences and pyrG sequences were integrated into the genome. The development of this pyrG transformation system should allow cloning of the aflatoxin-biosynthetic genes, which will be useful in studying the regulation of aflatoxin biosynthesis and may ultimately provide a means for controlling aflatoxin production in the field.

摘要

对于产黄曲霉毒素的寄生曲霉而言,缺乏高效的转化方法一直是在基因水平上研究黄曲霉毒素生物合成的主要制约因素。通过使用同源的pyrG基因,为寄生曲霉开发了一种转化系统,每微克DNA可产生30至50个稳定转化子。通过λ基因组DNA文库的原位噬菌斑杂交分离出寄生曲霉的pyrG基因。在亚硝基胍诱变后,通过在5-氟乳清酸上进行筛选,分离出寄生曲霉ATCC 36537的尿苷营养缺陷型菌株,该菌株在黄曲霉毒素生物合成中存在缺陷。通过检测细胞提取物将[14C]OMP转化为[14C]UMP的能力,检测出pyrG基因发生突变导致乳清苷单磷酸(OMP)脱羧酶活性丧失的分离株。用同源的pyrG基因转化寄生曲霉的pyrG原生质体,使真菌细胞恢复为原养型。对转化子克隆的细胞提取物进行酶分析表明,这些提取物具有将[14C]OMP转化为[14C]UMP的能力。对从转化子克隆中纯化的DNA进行Southern分析表明,pUC19载体序列和pyrG序列均已整合到基因组中。这种pyrG转化系统的开发应有助于克隆黄曲霉毒素生物合成基因,这将有助于研究黄曲霉毒素生物合成的调控,并最终可能为控制田间黄曲霉毒素的产生提供一种方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/733a/184948/5474a372448f/aem00092-0097-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/733a/184948/4744391b4f24/aem00092-0096-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/733a/184948/5474a372448f/aem00092-0097-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/733a/184948/4744391b4f24/aem00092-0096-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/733a/184948/5474a372448f/aem00092-0097-a.jpg

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