Extended nucleocapsid protein is cleaved from the Gag–Pol precursor of human immunodeficiency virus type 1

Author:

Chen Nissim1,Morag Abraham1,Almog Nava1,Blumenzweig Immanuel1,Dreazin Orna2,Kotler Moshe1

Affiliation:

1. Experimental Pathology Unit1 and Clinical Virology Unit2, The Hebrew University, Hadassah Medical School, PO Box 12272, Jerusalem 91120, Israel

2. National Public Health Laboratories, Ministry of Health, Israel3

Abstract

Human immunodeficiency virus type 1 Gag and Gag–Pol precursors are translated from an mRNA which is indistinguishable from the full-length genomic RNA. The ratio of Gag to Gag–Pol polyproteins is approximately 20:1 and is controlled by a frameshift of the reading frame, which takes place downstream of the p7 nucleocapsid (NC) in the N terminus of the p1 peptide. The viral precursors Gag and Gag–Pol are cleaved by the virus-encoded protease (PR) into the structural proteins, and into p6Pol, PR, reverse transcriptase and integrase. Due to the frameshift event, the cleavage site at the C terminus of NC coded in the Gag frame (ERQAN-FLGKI) changes either to ERQANFLRED or ERQANFFRED. The results presented in this report demonstrate that the NC released from the Gag–Pol precursor is 8 amino acid residues longer than the NC cleaved from the Gag polyprotein. Our results also show that truncated Gag–Pol precursors bearing cleavage site mutation at the NC/p6Pol, and/or p6Pol/PR junctions, undergo autoprocessing in bacterial and eukaryotic cells, indicating that PR is active when part of the precursor.

Publisher

Microbiology Society

Subject

Virology

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