analyses of in vivo interaction and mobility of two spliceosomal proteins using frap and bifc分析体内交互和移动两个使用收紧和bifc spliceosomal蛋白质.pdfVIP
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analyses of in vivo interaction and mobility of two spliceosomal proteins using frap and bifc分析体内交互和移动两个使用收紧和bifc spliceosomal蛋白质
Analyses of In Vivo Interaction and Mobility of Two
Spliceosomal Proteins Using FRAP and BiFC
Gul Shad Ali, K. V. S. K. Prasad¤a, M. Hanumappa¤b, A. S. N. Reddy*
Department of Biology and Program in Molecular Plant Biology, Colorado State University, Fort Collins, Colorado, United States of America
Abstract
U1-70K, a U1 snRNP-specific protein, and serine/arginine-rich (SR) proteins are components of the spliceosome and play
critical roles in both constitutive and alternative pre-mRNA splicing. However, the mobility properties of U1-70K, its in vivo
interaction with SR proteins, and the mobility of the U1-70K-SR protein complex have not been studied in any system. Here,
we studied the in vivo interaction of U1-70K with an SR protein (SR45) and the mobility of the U1-70K/SR protein complex
using bimolecular fluorescence complementation (BiFC) and fluorescence recovery after photobleaching (FRAP). Our results
show that U1-70K exchanges between speckles and the nucleoplasmic pool very rapidly and that this exchange is sensitive
to ongoing transcription and phosphorylation. BiFC analyses showed that U1-70K and SR45 interacted primarily in speckles
and that this interaction is mediated by the RS1 or RS2 domain of SR45. FRAP analyses showed considerably slower recovery
of the SR45/U1-70K complex than either protein alone indicating that SR45/U1-70K complexes remain in the speckles for a
longer duration. Furthermore, FRAP analyses with SR45/U1-70K complex in the presence of inhibitors of phosphorylation
did not reveal any significant change compared to control cells, suggesting that the mobility of the complex is not affected
by the status of protein phosphorylation. These results indicate that U1-70K, like SR splicing factors, moves rapidly in the
nucleus ensuring its availability at various sites of splicing. Furthermore, although it appears that U1-70K moves by diffusio
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