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在酿酒酵母中,Sit1与Aft1之间的物理相互作用通过抑制Sit1的蛋白质降解来上调FOB摄取活性。

Physical interaction between Sit1 and Aft1 upregulates FOB uptake activity by inhibiting protein degradation of Sit1 in Saccharomyces cerevisiae.

作者信息

Kang Chang-Min, Kang Suzie, Park Yong-Sung, Yun Cheol-Won

机构信息

School of Life Sciences and Biotechnology, Korea University, Anam-dong, Sungbuk-gu, Seoul 136-701, Republic of Korea.

School of Life Sciences and Biotechnology, Korea University, Anam-dong, Sungbuk-gu, Seoul 136-701, Republic of Korea

出版信息

FEMS Yeast Res. 2015 Nov;15(7). doi: 10.1093/femsyr/fov080. Epub 2015 Aug 30.

DOI:10.1093/femsyr/fov080
PMID:26323600
Abstract

Previously, we reported that Aft1 regulates Sit1 by modulating the ubiquitination of Sit1 in Saccharomyces cerevisiae. Here, we report the function of the physical interaction between Sit1 and Aft1 in ferrioxamine B (FOB) uptake. The interaction between Sit1 and Aft1 induced protein localization of Sit1 to the plasma membrane, and more Sit1 was detected in the plasma membrane when Sit1 and Aft1 were coexpressed compared with Sit1 expression alone. The MSN5-deletion mutant, which failed to translocate Aft1 to the cytosolic compartment, showed lower FOB uptake activity than the wild type. However, higher free iron uptake activity was detected in the MSN5-deletion mutant. Furthermore, the strain transformed with AFT1-1(up) plasmid, which failed to regulate Aft1 via iron concentration and accumulated Aft1 in the nucleus, showed lower FOB uptake activity. The Aft1 Y179F mutant, which contained a tyrosine residue that was changed to phenylalanine, failed to interact physically with Sit1 and showed more degradation of the Sit1 and, ultimately, lower FOB uptake activity. Additionally, we found that MG132 and PMSF, which are inhibitors of proteasomes and serine proteases, respectively, increased the Sit1 protein level. Taken together, these results suggest that the protein-protein interaction between Sit1 and Aft1 is an important factor in the FOB uptake activity of Sit1.

摘要

此前,我们报道过在酿酒酵母中,Aft1通过调节Sit1的泛素化来调控Sit1。在此,我们报道Sit1与Aft1之间的物理相互作用在高铁载体B(FOB)摄取中的功能。Sit1与Aft1之间的相互作用促使Sit1蛋白定位于质膜,与单独表达Sit1相比,当Sit1和Aft1共表达时,在质膜中检测到更多的Sit1。MSN5缺失突变体无法将Aft1转运至胞质区室,其FOB摄取活性低于野生型。然而,在MSN5缺失突变体中检测到更高的游离铁摄取活性。此外,用AFT1 - 1(up)质粒转化的菌株无法通过铁浓度调节Aft1并使Aft1在细胞核中积累,其FOB摄取活性较低。Aft1 Y179F突变体中一个酪氨酸残基被替换为苯丙氨酸,它无法与Sit1发生物理相互作用,且Sit1降解更多,最终FOB摄取活性较低。此外,我们发现蛋白酶体抑制剂MG132和丝氨酸蛋白酶抑制剂PMSF分别提高了Sit1蛋白水平。综上所述,这些结果表明Sit1与Aft1之间的蛋白质 - 蛋白质相互作用是Sit1的FOB摄取活性的一个重要因素。

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