Molecular Characterization of Proteolytic Processing of the Pol Proteins of Human Foamy Virus Reveals Novel Features of the Viral Protease

Author:

Pfrepper Klaus-Ingmar1,Rackwitz Hans-Richard2,Schnölzer Martina3,Heid Hans2,Löchelt Martin1,Flügel Rolf M.1

Affiliation:

1. Abteilungen Retroviral Gene Expression, Research Program Applied Tumorvirology,1

2. Cell Biology, Research Program Cell Differentiation and Carcinogenesis,2 and

3. Central Protein Analysis Group,3 German Cancer Research Center, 69009 Heidelberg, Federal Republic of Germany

Abstract

ABSTRACT Spumaviruses, or foamy viruses, express a pol -specific transcript that codes for a Pol polyprotein that consists of the protease, reverse transcriptase, ribonuclease H, and the integrase domains. To delineate the proteolytic cleavage sites between the Pol subdomains, recombinant human foamy virus (HFV) Pol proteins were expressed, purified by affinity chromatography, and subjected to either HFV protease assays or autocatalytic processing. In control experiments, HFV protease-deficient mutant proteins in which the active site Asp was replaced by an Ala residue were used to rule out unspecific processing by nonviral proteases. Specific proteolytic cleavage products were isolated, and the cleavage sites were analyzed by amino acid sequencing. Peptides spanning the resulting cleavage sites were chemically synthesized and assayed with HFV protease, and the cleaved peptides were subjected to mass spectrometry. The cleavage site sequences obtained were in complete agreement with the amino-terminal sequences from amino acid sequencing of authentic cleavage products of the HFV Pol proteins. Analysis by fast-protein liquid chromatography of a short version of the active HFV protease revealed that the enzyme predominantly formed dimeric molecules.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

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