Analysis and Molecular Determinants of HIV RNase H Cleavage Specificity at the PPT/U3 Junction

Álvarez, Mar and Sapena-Ventura, Enrique and Luczkowiak, Joanna and Martín-Alonso, Samara and Menéndez-Arias, Luis (2021) Analysis and Molecular Determinants of HIV RNase H Cleavage Specificity at the PPT/U3 Junction. Viruses, 13 (1). p. 131. ISSN 1999-4915

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Abstract

HIV reverse transcriptases (RTs) convert viral genomic RNA into double-stranded DNA. During reverse transcription, polypurine tracts (PPTs) resilient to RNase H cleavage are used as primers for plus-strand DNA synthesis. Nonnucleoside RT inhibitors (NNRTIs) can interfere with the initiation of plus-strand DNA synthesis by enhancing PPT removal, while HIV RT connection subdomain mutations N348I and N348I/T369I mitigate this effect by altering RNase H cleavage specificity. Now, we demonstrate that among approved nonnucleoside RT inhibitors (NNRTIs), nevirapine and doravirine show the largest effects. The combination N348I/T369I in HIV-1BH10 RT has a dominant effect on the RNase H cleavage specificity at the PPT/U3 site. Biochemical studies showed that wild-type HIV-1 and HIV-2 RTs were able to process efficiently and accurately all tested HIV PPT sequences. However, the cleavage accuracy at the PPT/U3 junction shown by the HIV-2EHO RT was further improved after substituting the sequence YQEPFKNLKT of HIV-1BH10 RT (positions 342–351) for the equivalent residues of the HIV-2 enzyme (HQGDKILKV). Our results highlight the role of β-sheets 17 and 18 and their connecting loop (residues 342–350) in the connection subdomain of the large subunit, in determining the RNase H cleavage window of HIV RTs.

Item Type: Article
Uncontrolled Keywords: HIV; reverse transcriptase; antiretroviral drug resistance; DNA synthesis; doravirine; RNase H
Subjects: e-Archives > Medical Science
Depositing User: Managing Editor
Date Deposited: 17 Jan 2023 11:44
Last Modified: 29 Jun 2024 11:30
URI: http://ebooks.abclibraries.com/id/eprint/127

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