首页> 美国卫生研究院文献>Genetics >zds1 a Novel Gene Encoding an Ortholog of Zds1 and Zds2 Controls Sexual Differentiation Cell Wall Integrity and Cell Morphology in Fission Yeast
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zds1 a Novel Gene Encoding an Ortholog of Zds1 and Zds2 Controls Sexual Differentiation Cell Wall Integrity and Cell Morphology in Fission Yeast

机译:zds1一种编码Zds1和Zds2直系同源物的新型基因可控制裂变酵母中的性别分化细胞壁完整性和细胞形态

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摘要

While screening for genes that reverse the sporulation-deficient phenotype of the ras1Δ diploid Schizosaccharomyces pombe strain, we identified zds1. This gene shares sequence homology with the ZDS1 and ZDS2 genes from Saccharomyces cerevisiae, which appear to be involved in multiple cellular events. Expression of Zds1 in ras1Δ diploid cells elevated their sporulation rate from 0.3 to 11.2%. Expression of the Zds1 C-terminal region increased the sporulation rate further (to 21.9%) while introduction of the Zds1 N-terminal region had no effect. zds1 expression did not induce sporulation in strains with mutations in genes participating in the downstream MAP kinase cascade. The zds1-disrupted strain is sensitive to CaCl2, and this effect is suppressed by the C-terminal region of Zds1. The growth of the zds1Δ strain is markedly inhibited by cold temperatures, while its viability decreased in the stationary phase. Moreover, the zds1Δ strain is round in shape and very sensitive to zymolyase, and its cell wall becomes thicker than that of wild type. Thus, zds1 must be required to maintain cell wall integrity. The Zds1–GFP fusion protein localized to the cytosol, the septum, and the cell cortex. Its localization in the septum was dependent on its C-terminal region. Overexpression of the C-terminal region of Zds1 induced multi-septa and abnormal zygotes. We propose that the C-terminal region is the functional domain of Zds1 while the N-terminal region is a negative regulatory region. Thus, Zds1 is involved in multiple cellular events in fission yeast, including sexual differentiation, Ca2+ tolerance, cell wall integrity, viability in the stationary phase, and cell morphology.
机译:在筛选可逆转ras1Δ二倍体Schizosaccharomyces pombe菌株孢子形成缺陷表型的基因时,我们鉴定了zds1。该基因与酿酒酵母的ZDS1和ZDS2基因具有序列同源性,似乎与多种细胞事件有关。 Zds1在ras1Δ二倍体细胞中的表达将其孢子形成率从0.3%提高到11.2%。 Zds1 C末端区域的表达进一步增加了孢子形成率(至21.9%),而引入Zds1 N末端区域没有影响。 zds1表达不会在参与下游MAP激酶级联反应的基因突变的菌株中诱导孢子形成。破坏zds1的菌株对CaCl2敏感,并且这种作用被Zds1的C端区域抑制。 zds1Δ菌株的生长受到低温的明显抑制,而其活力在固定相中降低。而且,zds1Δ菌株是圆形的并且对酶解酶非常敏感,并且其细胞壁比野生型的细胞壁更厚。因此,必须要求zds1才能维持细胞壁完整性。 Zds1-GFP融合蛋白位于细胞质,隔膜和细胞皮层。其在隔膜中的定位取决于其C端区域。 Zds1的C端区域的过度表达诱导多隔和合子异常。我们建议C末端区域是Zds1的功能域,而N末端区域是负调控区域。因此,Zds1参与了裂变酵母中的多种细胞事件,包括性别分化,Ca 2 + 耐受性,细胞壁完整性,固定相的生存能力以及细胞形态。

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