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细胞器内伴侣蛋白应对应激诱导的蛋白质解折叠的能力比较。

Comparison of intra-organellar chaperone capacity for dealing with stress-induced protein unfolding.

作者信息

Hageman Jurre, Vos Michel J, van Waarde Maria A W H, Kampinga Harm H

机构信息

Department of Cell Biology, Section of Radiation and Stress Cell Biology, University Medical Center Groningen, University of Groningen, Groningen, The Netherlands.

出版信息

J Biol Chem. 2007 Nov 23;282(47):34334-45. doi: 10.1074/jbc.M703876200. Epub 2007 Sep 17.

DOI:10.1074/jbc.M703876200
PMID:17875648
Abstract

Molecular chaperones are essential for cells to prevent that partially unfolded proteins form non-functional, toxic aggregates. This requirement is increased when cells experience protein unfolding stresses and such could affect all compartments in the eukaryotic cell. Whether all organelles are equipped with comparable chaperone capacities is largely unknown, mainly due to the lack of suitable reporters that allow such a comparison. Here we describe the development of fluorescent luciferase reporters that are sorted to various cellular locations (nucleus, cytoplasm, endoplasmic reticulum, and peroxisomes) and that differ minimally in their intrinsic thermal stability properties. When heating living cells, the rate of inactivation was most rapid for the nuclear-targeted luciferase, indicating that the nucleus is the most sensitive organelle toward heat-induced denaturing stress. Post-heat re-activation, however, occurred at equal kinetics irrespective of luciferase localization. Also, induction of thermotolerance by a priming heat treatment, that coordinately up-regulates all heat-inducible chaperones, resulted in a transient heat resistance of the luciferase in all organelles in a comparable manner. Overexpression of the main heat-inducible Hsp70 family member, HspA1A, protected only the cytosolic and nuclear, but not the other luciferases. Together, our data suggest that in each compartment investigated, including the peroxisome in which so far no chaperones could be detected, chaperone machines are present and can be induced with activities similar to those present in the cytosolic/nuclear compartment.

摘要

分子伴侣对于细胞防止部分未折叠的蛋白质形成无功能的毒性聚集体至关重要。当细胞经历蛋白质解折叠应激时,这种需求会增加,并且这可能会影响真核细胞的所有区室。目前很大程度上不清楚所有细胞器是否都具备相当的伴侣蛋白能力,主要是因为缺乏能够进行这种比较的合适报告分子。在这里,我们描述了荧光素酶报告分子的开发,这些报告分子被分选到不同的细胞位置(细胞核、细胞质、内质网和过氧化物酶体),并且它们的内在热稳定性特性差异最小。当加热活细胞时,核靶向荧光素酶的失活速率最快,这表明细胞核是对热诱导变性应激最敏感的细胞器。然而,热后重新激活以相同的动力学发生,与荧光素酶的定位无关。此外,通过引发热处理诱导热耐受性,协同上调所有热诱导伴侣蛋白,以类似的方式导致所有细胞器中的荧光素酶产生短暂的耐热性。主要热诱导的Hsp70家族成员HspA1A的过表达仅保护细胞质和细胞核中的荧光素酶,而不保护其他荧光素酶。总之,我们的数据表明,在所研究的每个区室中,包括迄今为止未检测到伴侣蛋白的过氧化物酶体,都存在伴侣蛋白机器,并且可以被诱导,其活性与细胞质/细胞核区室中的活性相似。