Sharp Z Dave, Stenoien David L, Mancini Maureen G, Ouspenski Ilia I, Mancini Michael A
Department of Molecular and Cellular Biology, Baylor College of Medicine, Houston, Texas 77003, USA.
J Cell Biochem. 2004 Jul 1;92(4):664-78. doi: 10.1002/jcb.20028.
Pit-1, a POU-class nuclear DNA-binding transcription factor, specifies three of the parenchymal cell types in anterior pituitary ontogeny. Using fluorescent fusions and live cell imaging, we have compared the dynamic behavior of wild-type and inactivating Pit-1 point mutations. Fluorescence recovery after photobleaching (FRAP) and real-time extraction data indicate that wild-type Pit-1 has a dynamic mobility profile, with t(1/2s) approximately 5-7 s when expressed from low to high amounts, respectively. Biochemically, Pit-1 is approximately 50% retained according to direct observation during extraction, indicating a dynamic interaction with nuclear structure. An analysis of transiently expressed Pit-1 carrying two different debilitating mutations reveals that they translocate normally to the nucleus, but exhibit two different levels of mobility, both clearly distinguishable from wild-type Pit-1. At low expression levels, the t(1/2s) of Pit(W261C) and Pit(A158P) are extremely rapid (0.3 and 0.6 s t(1/2s), respectively). At higher expression levels, unlike wild-type Pit-1, both mutant proteins become immobilized and insoluble, and fractionate completely with the insoluble nuclear matrix. Relative to wild-type, over expression of mutated Pit-1 elicits a nuclear stress response indicated by increased levels of heat shock inducible heat shock protein 70 (Hsp70), and reorganization of heat shock factor-1. The decreased mobility of Pit(A158P) relative to Pit(W261C) at low expression levels correlates with its ability to partially activate when expressed at low levels and its ability to bind cognate DNA. At high expression levels, lower Pit(A158P) activation correlates with its immobilization and insolubility. These data suggest a link between specific rates of intranuclear mobility and Pit-1 transcription function, perhaps to insure sufficient interactions with chromatin, or in the case of non-DNA binding Pit-1, interaction as a repressor. These data imply inactivating mutations can lead to an intranuclear sorting away from transcription related pathways, and at least in part to a misfolded protein pathway. Taken together, caution is suggested when interpreting point (or other) mutational analyses of transactivator function, as new compartmentation, especially in the context of expression levels, may cloud the distinction between defining functional molecular domains and intranuclear processing of misfolded proteins.
Pit-1是一种POU类核DNA结合转录因子,它决定了垂体前叶发育过程中三种实质细胞类型。我们使用荧光融合蛋白和活细胞成像技术,比较了野生型和失活的Pit-1点突变体的动态行为。光漂白后荧光恢复(FRAP)和实时提取数据表明,野生型Pit-1具有动态迁移特性,当从低表达量到高表达量表达时,其半衰期(t(1/2s))分别约为5 - 7秒。生化分析表明,在提取过程中直接观察到约50%的Pit-1被保留,这表明它与核结构存在动态相互作用。对携带两种不同失活突变的瞬时表达的Pit-1进行分析发现,它们能正常转运到细胞核,但表现出两种不同水平的迁移率,且都与野生型Pit-1明显不同。在低表达水平时,Pit(W261C)和Pit(A158P)的半衰期(t(半))极快(分别为0.3秒和0.6秒)。在高表达水平时,与野生型Pit-1不同,这两种突变蛋白都变得固定且不溶,并完全与不溶性核基质分离。相对于野生型,突变型Pit-1的过表达引发了核应激反应,表现为热休克诱导型热休克蛋白70(Hsp70)水平升高以及热休克因子-1的重新组织。在低表达水平时,Pit(A158P)相对于Pit(W261C)迁移率降低,这与其在低表达时部分激活的能力及其结合同源DNA的能力相关。在高表达水平时,Pit(A158P)较低的激活能力与其固定化和不溶性相关。这些数据表明核内迁移的特定速率与Pit-1转录功能之间存在联系,可能是为了确保与染色质有足够的相互作用,或者对于非DNA结合的Pit-1来说,是作为一种阻遏物进行相互作用。这些数据表明失活突变可导致在核内从转录相关途径中分离出来,至少部分导致错误折叠蛋白途径。综上所述,在解释反式激活因子功能的点突变(或其他)分析时应谨慎,因为新的区室化,特别是在表达水平的背景下,可能会模糊定义功能分子结构域和错误折叠蛋白的核内加工之间的区别。
