Abstract

Viruses have evolved intricate mechanisms for hijacking cellular resources to replicate and spread. Over the past two decades, great progress has been made in identifying hundreds of cellular factors involved in HIV transcription and describing their critical importance in AIDS pathogenesis. However, there is currently a dearth of information regarding how these protein complexes communicate to sustain active transcription, and how their deregulation leads to the establishment of latency. The identification of new regulatory factors, their assembly and function will provide not only mechanistic insights but it will elucidate novel candidate targets for HIV eradication strategies. This research project aims at further investigating the role of Tat and novel host co-factors in HIV transcription and their role in promoting viral latency. Tat activates the transition into elongation by transferring P-TEF from the inhibitory, promoter-bound 7SK snRNP to the TAR element on nascent viral pre-mRNAs. In this model, Tat recruits the PPM1G phosphatase to the promoter-bound 7SK snRNP to dephosphorylate the T loop of the P-TEFb kinase thereby locally releasing P-TEFb to activate transcription elongation. However, detailed dissection of the steps of: (i) 7SK snRNP recruitment to the HIV promoter to restrict transcription elongation, (ii) assembly of the Tat-PPM1G-7SK complex to release P-TEFb, and (iii) the role of PPM1G in sustaining viral transcription, is still incomplete. This research project will use a wide- range of approaches to elucidate the mechanism by which the 7SK snRNP is recruited to the HIV promoter and how Tat assembles with PPM1G to capture P-TEFb from the snRNP to activate viral transcription. The work proposed builds on a recent publication and a novel set of preliminary data that identified: (i) KAP1/TRIM28 as a possible factor that recruits the 7SK snRNP to the HIV promoter to restrict proviral transcription, and (ii) novel features of the assembly of PPM1G into the 7SK snRNP (to release P-TEFb and activate HIV transcription). Given that these Tat co-factors restrict proviral transcription, they emerge as key candidates for rationale HIV eradication strategies. The project will be conducted at U.T. Southwestern Medical Center, which has state-of-the-art technologies and a very rich atmosphere of collaborators in fields other than virology. An ongoing collaboration with Dr V. Planelles (University of Utah) will be critical to provide a mechanistic understanding of latency in primary cells. Collectively, these discoveries will elucidate the role of these cellular factors in proviral transcription and latency, and will provid novel opportunities to reactivate latent HIV.

Public Health Relevance

This project will combine a wide-range of approaches to further understand the process of HIV transcription and latency. We aim to precisely delineate how Tat exploits novel host co-factors for HIV transcription activation and how deregulation of these processes leads to transcriptional silencing and entry into latency, a barrier for HIV eradication. This information will aid in an incremental understanding of Tat activation and will provide novel therapeutic opportunities towards efforts for a functional cure.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI114362-03
Application #
9188800
Study Section
AIDS Molecular and Cellular Biology Study Section (AMCB)
Program Officer
Kuo, Lillian S
Project Start
2015-01-01
Project End
2019-12-31
Budget Start
2017-01-01
Budget End
2017-12-31
Support Year
3
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
University of Texas Sw Medical Center Dallas
Department
Microbiology/Immun/Virology
Type
Schools of Medicine
DUNS #
800771545
City
Dallas
State
TX
Country
United States
Zip Code
75390

  Publications

Faust, Tyler B; Li, Yang; Bacon, Curtis W et al. (2018) The HIV-1 Tat protein recruits a ubiquitin ligase to reorganize the 7SK snRNP for transcriptional activation. Elife 7:
Bacon, Curtis W; D'Orso, Iván (2018) CDK9: a signaling hub for transcriptional control. Transcription :1-19
Guzman, Carlos; D'Orso, Iván (2017) CIPHER: a flexible and extensive workflow platform for integrative next-generation sequencing data analysis and genomic regulatory element prediction. BMC Bioinformatics 18:363
Ma, Zheng; Fung, Victor; D'Orso, Iván (2017) Tandem Affinity Purification of Protein Complexes from Eukaryotic Cells. J Vis Exp :
D'Orso, Iván (2016) 7SKiing on chromatin: Move globally, act locally. RNA Biol 13:545-53
McNamara, Ryan P; Bacon, Curtis W; D'Orso, Iván (2016) Transcription elongation control by the 7SK snRNP complex: Releasing the pause. Cell Cycle 15:2115-2123
McNamara, Ryan P; Guzman, Carlos; Reeder, Jonathan E et al. (2016) Genome-wide analysis of KAP1, the 7SK snRNP complex, and RNA polymerase II. Genom Data 7:250-5
Gudipaty, Swapna Aravind; D'Orso, Iván (2016) Functional interplay between PPM1G and the transcription elongation machinery. RNA Dis 3:
McNamara, Ryan P; Reeder, Jonathan E; McMillan, Elizabeth A et al. (2016) KAP1 Recruitment of the 7SK snRNP Complex to Promoters Enables Transcription Elongation by RNA Polymerase II. Mol Cell 61:39-53
Gudipaty, Swapna Aravind; McNamara, Ryan P; Morton, Emily L et al. (2015) PPM1G Binds 7SK RNA and Hexim1 To Block P-TEFb Assembly into the 7SK snRNP and Sustain Transcription Elongation. Mol Cell Biol 35:3810-28

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