Skibinski Gregory A, Boyd Lynn
Department of Biological Sciences, University of Alabama in Huntsville, Huntsville AL 35899, USA.
BMC Cell Biol. 2012 Apr 11;13:10. doi: 10.1186/1471-2121-13-10.
Protein misfolding and subsequent aggregation are hallmarks of several human diseases. The cell has a variety of mechanisms for coping with misfolded protein stress, including ubiquitin-mediated protein degradation. In fact, the presence of ubiquitin at protein aggregates is a common feature of protein misfolding diseases. Ubiquitin conjugating enzymes (UBCs) are part of the cascade of enzymes responsible for the regulated attachment of ubiquitin to protein substrates. The specific UBC used during ubiquitination can determine the type of polyubiquitin chain linkage, which in turn plays an important role in determining the fate of the ubiquitinated protein. Thus, UBCs may serve an important role in the cellular response to misfolded proteins and the fate of protein aggregates.
The Q82 strain of C. elegans harbors a transgene encoding an aggregation prone tract of 82 glutamine residues fused to green fluorescent protein (Q82::GFP) that is expressed in the body wall muscle. When measured with time-lapse microscopy in young larvae, the initial formation of individual Q82::GFP aggregates occurs in approximately 58 minutes. This process is largely unaffected by a mutation in the C. elegans E1 ubiquitin activating enzyme. RNAi of ubc-22, a nematode homolog of E2-25K, resulted in higher pre-aggregation levels of Q82::GFP and a faster initial aggregation rate relative to control. Knockdown of ubc-1 (RAD6 homolog), ubc-13, and uev-1 did not affect the kinetics of initial aggregation. However, RNAi of ubc-13 decreases the rate of secondary growth of the aggregate. This result is consistent with previous findings that aggregates in young adult worms are smaller after ubc-13 RNAi. mCherry::ubiquitin becomes localized to Q82::GFP aggregates during the fourth larval (L4) stage of life, a time point long after most aggregates have formed. FLIP and FRAP analysis indicate that mCherry::ubiquitin is considerably more mobile than Q82::GFP within aggregates.
These data indicate that initial formation of Q82::GFP aggregates in C. elegans is not directly dependent on ubiquitination, but is more likely a spontaneous process driven by biophysical properties in the cytosol such as the concentration of the aggregating species. The effect of ubiquitination appears to be most significant in later, secondary aggregate growth.
蛋白质错误折叠及随后的聚集是多种人类疾病的标志。细胞具有多种应对错误折叠蛋白应激的机制,包括泛素介导的蛋白质降解。事实上,蛋白质聚集体中泛素的存在是蛋白质错误折叠疾病的一个共同特征。泛素结合酶(UBCs)是负责将泛素调节性连接到蛋白质底物的酶级联反应的一部分。泛素化过程中使用的特定UBC可以决定多聚泛素链的连接类型,这反过来又在决定泛素化蛋白质的命运中起重要作用。因此,UBCs可能在细胞对错误折叠蛋白的反应以及蛋白质聚集体的命运中发挥重要作用。
秀丽隐杆线虫的Q82菌株携带一个转基因,该转基因编码一个与绿色荧光蛋白融合的82个谷氨酰胺残基的易聚集区(Q82::GFP),其在体壁肌肉中表达。当在幼虫中用延时显微镜测量时,单个Q82::GFP聚集体的初始形成大约发生在58分钟内。这个过程在很大程度上不受秀丽隐杆线虫E1泛素激活酶突变的影响。线虫E2-25K同源物ubc-22的RNA干扰导致Q82::GFP的聚集前水平更高,并且相对于对照,初始聚集速率更快。ubc-1(RAD6同源物)、ubc-13和uev-1的敲低不影响初始聚集的动力学。然而,ubc-13的RNA干扰降低了聚集体二次生长的速率。这一结果与之前的研究结果一致,即在ubc-13 RNA干扰后,年轻成虫中的聚集体更小。在生命的第四幼虫期(L4),mCherry::泛素定位于Q82::GFP聚集体,这是在大多数聚集体形成后的一个时间点。荧光漂白恢复(FLIP)和荧光漂白后恢复(FRAP)分析表明,mCherry::泛素在聚集体中的移动性比Q82::GFP大得多。
这些数据表明,秀丽隐杆线虫中Q82::GFP聚集体的初始形成不直接依赖于泛素化,而更可能是由细胞质中的生物物理性质(如聚集物种的浓度)驱动的自发过程。泛素化的作用似乎在后期聚集体的二次生长中最为显著。
Zotero 插件
