Abstract EN:

Transcription of RNA polymerase II (RNAPII) is a highly complex procedure, including initiation, promoter escape, elongation and termination. Each step of transcription is regulated by a variety of cis-elements and trans-factors. Maturation of RNAPII transcripts is also a complicated course consisting of transcript capping, splicing and 3’ end processing. It is widely accepted that RNAPII transcription and its RNA processing are interactional and different processes of RNAPII transcript maturation influence each other. In the attempt of finding the non-coding RNAs that can regulate the activity of RNAPII in mammals, we found that U1 snRNA is associated with RNAPII no matter if RNAPII is transcribing or not. Moreover, using fluorescence microscopy, we showed that the interaction between U1 snRNA and RNAPII is independent on splicing, which is the main function of U1 snRNA. During the investigation of the effect of RNAPII on transcript maturation, I focused on post-translational phosphorylation of the carboxyl-terminal domain of RNAPII, which is the unique domain of RNAPII in all RNAPI, II and III. I found that the phosphorylation of CTD serine 2 residues is required for constitutive splicing as well as 3’ end processing. I also provided the evidence to show the effect of splicing on 3’ end processing via the splicing factor U2AF65. Furthermore, I showed the effect of CTD serine 2 residue phosphorylation on alternative splicing and the recruitment of TAF15, PSF and P54 to the transcription sites. Finally, I summarized the unknown points in my study and proposed the perspective.