Deletion of PIN4 Suppresses the Protein Transport Defects Caused by sec12-4 Mutation in Saccharomyces cerevisiae.

Pub Date : 2020-01-01 Epub Date: 2020-09-15 DOI:10.1159/000509633
Akiko Murakami-Sekimata, Masayuki Sekimata, Natsumi Sato, Yuto Hayasaka, Akihiko Nakano
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Abstract

Newly synthesized secretory proteins are released into the lumen of the endoplasmic reticulum (ER). The secretory proteins are surrounded by coat protein complex II (COPII) vesicles, and transported from the ER and reach their destinations through the Golgi apparatus. Sec12p is a guanine nucleotide exchange factor for Sar1p, which initiates COPII vesicle budding from the ER. The activation of Sar1p by Sec12p and the subsequent COPII coat assembly have been well characterized, but the events that take place upstream of Sec12p remain unclear. In this study, we isolated the novel extragenic suppressor of sec12-4, PIN4/MDT1, a cell cycle checkpoint target. A yeast two-hybrid screening was used to identify Pin4/Mdt1p as a binding partner of the casein kinase I isoform Hrr25p, which we have previously identified as a modulator of Sec12p function. Deletion of PIN4 suppressed both defects of temperature-sensitive growth and the partial protein transport observed in sec12-4 mutants. The results of this study suggest that Pin4p provides novel aspects of Sec12p modulations.

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PIN4缺失抑制酿酒酵母sec12-4突变引起的蛋白质转运缺陷
新合成的分泌蛋白被释放到内质网(ER)的管腔。分泌蛋白被外壳蛋白复合物II (COPII)囊泡包围,从内质网运输并通过高尔基体到达目的地。Sec12p是Sar1p的鸟嘌呤核苷酸交换因子,Sar1p启动内质网的COPII囊泡出芽。Sar1p被Sec12p激活以及随后的COPII外壳组装已经被很好地表征,但发生在Sec12p上游的事件仍不清楚。在这项研究中,我们分离了sec12-4的新的外基因抑制因子,PIN4/MDT1,一个细胞周期检查点靶点。通过酵母双杂交筛选,我们确定了Pin4/Mdt1p是酪蛋白激酶I异构体Hrr25p的结合伙伴,我们之前已经确定了Hrr25p是Sec12p功能的调节因子。在sec12-4突变体中,PIN4的缺失抑制了温度敏感生长缺陷和部分蛋白质转运。本研究的结果表明,Pin4p提供了Sec12p调制的新方面。
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