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里氏木霉原生质体融合,利用未成熟分生孢子。

Protoplast Fusion of Trichoderma reesei, Using Immature Conidia.

机构信息

Department of Fermentation Technology, Faculty of Engineering, Osaka University, Yamada-oka, Suita-shi, Osaka 565, Japan.

出版信息

Appl Environ Microbiol. 1984 Feb;47(2):363-8. doi: 10.1128/aem.47.2.363-368.1984.

Abstract

Protoplast fusion of strains derived from Trichoderma reesei QM9414 and QM9136 and the segregation of the resulting fusants were studied. Combinations of protoplasts prepared from young conidia with double amino acid requirements, one of which was a common requirement and the other uncommon, were fused in the presence of polyethylene glycol 6000. Fusants were selected as regenerant colonies requiring only the commonly deficient amino acid. The frequency of fusion was 0.9 x 10 to 4.0 x 10 for the starting conidia and 3.0 x 10 to 4.9 x 10 for the regenerated protoplasts, which was significantly higher than the expected reversion frequencies by mutation. Conidia generated on the fusant colonies showed diverse phenotypes, i.e., parental types (40 to 80%) and nonparental types (20 to 60%). Colonies developed from single conidia of the nonparental phenotype contained special spots called "knobs" that have a higher density of mycelia. The phenotype of the knobs was again varied among prototrophs, parental types, and recombinant types; and their traits were inherited stably. The phenotype of the mycelia in the nonknob part was essentially the same as that of the original conidia and again formed knobs in colonies upon transfer of a piece of mycelia to a fresh medium. The conidial DNA content of the knob clone was almost the same as that of the parents, but that of the fusants was 1.2 to 2.0 times higher than that of the parents. From these results, we conclude that knobs are the segregants from the fusants. One knob clone showed twice the carboxymethyl cellulose hydrolyzing activity of the parents, suggesting the possibility of breeding T. reesei cells by the protoplast fusion technique.

摘要

对来源于里氏木霉 QM9414 和 QM9136 的菌株的原生质体融合和融合子的分离进行了研究。在聚乙二醇 6000 的存在下,将具有双重氨基酸需求的幼龄分生孢子制备的原生质体进行融合,其中一种是常见需求,另一种是不常见需求。融合子被选为仅需要常见缺乏的氨基酸的再生菌落。融合的频率为起始分生孢子的 0.9×10 至 4.0×10,再生原生质体的 3.0×10 至 4.9×10,明显高于突变引起的预期回复频率。融合子菌落上产生的分生孢子表现出不同的表型,即亲本类型(40%至 80%)和非亲本类型(20%至 60%)。非亲本表型单分生孢子产生的菌落含有称为“瘤”的特殊斑点,其菌丝密度更高。瘤的表型在营养缺陷型中再次表现出多样性,包括亲本类型和重组类型;它们的特性稳定遗传。无瘤部分的菌丝表型与原始分生孢子基本相同,并且在将一段菌丝转移到新鲜培养基上时再次在菌落中形成瘤。瘤克隆的分生孢子 DNA 含量几乎与亲本相同,但融合子的 DNA 含量是亲本的 1.2 至 2.0 倍。根据这些结果,我们得出结论,瘤是融合子的分离物。一个瘤克隆显示出亲本两倍的羧甲基纤维素水解活性,这表明通过原生质体融合技术培育里氏木霉细胞的可能性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/99eb/239675/361eb4d044ae/aem00159-0151-a.jpg

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