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酿酒酵母中双态性的调控:新型蛋白激酶同源物Elm1p和蛋白磷酸酶2A的作用。

Regulation of dimorphism in Saccharomyces cerevisiae: involvement of the novel protein kinase homolog Elm1p and protein phosphatase 2A.

作者信息

Blacketer M J, Koehler C M, Coats S G, Myers A M, Madaule P

机构信息

Department of Biochemistry and Biophysics, Iowa State University, Ames 50011.

出版信息

Mol Cell Biol. 1993 Sep;13(9):5567-81. doi: 10.1128/mcb.13.9.5567-5581.1993.

Abstract

The Saccharomyces cerevisiae genes ELM1, ELM2, and ELM3 were identified on the basis of the phenotype of constitutive cell elongation. Mutations in any of these genes cause a dimorphic transition to a pseudohyphal growth state characterized by formation of expanded, branched chains of elongated cells. Furthermore, elm1, elm2, and elm3 mutations cause cells to grow invasively under the surface of agar medium. S. cerevisiae is known to be a dimorphic organism that grows either as a unicellular yeast or as filamentous cells termed pseudohyphae; although the yeast-like form usually prevails, pseudohyphal growth may occur during conditions of nitrogen starvation. The morphologic and physiological properties caused by elm1, elm2, and elm3 mutations closely mimic pseudohyphal growth occurring in conditions of nitrogen starvation. Therefore, we propose that absence of ELM1, ELM2, or ELM3 function causes constitutive execution of the pseudohyphal differentiation pathway that occurs normally in conditions of nitrogen starvation. Supporting this hypothesis, heterozygosity at the ELM2 or ELM3 locus significantly stimulated the ability to form pseudohyphae in response to nitrogen starvation. ELM1 was isolated and shown to code for a novel protein kinase homolog. Gene dosage experiments also showed that pseudohyphal differentiation in response to nitrogen starvation is dependent on the product of CDC55, a putative B regulatory subunit of protein phosphatase 2A, and a synthetic phenotype was observed in elm1 cdc55 double mutants. Thus, protein phosphorylation is likely to regulate differentiation into the pseudohyphal state.

摘要

酿酒酵母基因ELM1、ELM2和ELM3是根据组成型细胞伸长的表型鉴定出来的。这些基因中的任何一个发生突变都会导致双态转变为假菌丝生长状态,其特征是形成伸长细胞的扩展分支链。此外,elm1、elm2和elm3突变会使细胞在琼脂培养基表面下侵入性生长。已知酿酒酵母是一种双态生物,它可以以单细胞酵母或称为假菌丝的丝状细胞形式生长;尽管酵母样形式通常占主导,但在氮饥饿条件下可能会出现假菌丝生长。由elm1、elm2和elm3突变引起的形态学和生理学特性与氮饥饿条件下发生的假菌丝生长非常相似。因此,我们提出ELM1、ELM2或ELM3功能的缺失会导致在氮饥饿条件下正常发生的假菌丝分化途径的组成型执行。支持这一假设的是,ELM2或ELM3位点的杂合性显著刺激了对氮饥饿形成假菌丝的能力。ELM1被分离出来并显示编码一种新型蛋白激酶同源物。基因剂量实验还表明,对氮饥饿的假菌丝分化依赖于蛋白磷酸酶2A的假定B调节亚基CDC55的产物,并且在elm1 cdc55双突变体中观察到了合成表型。因此,蛋白质磷酸化可能调节向假菌丝状态的分化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4238/360278/41fa8f6efea1/molcellb00021-0451-a.jpg

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