Abstract

Interactions of viral proteins play an important role in the virus life cycle, especially in capsid assembly. Andean potato mottle comovirus (APMoV) is a plant RNA virus with a virion formed by two coat proteins (CP42 and CP22). Both APMoV coat protein open reading frames were cloned into pGBT9 and pGAD10, two-hybrid system vectors. HF7c yeast cells transformed with the p9CP42 construct grew on yeast dropout selection media lacking tryptophan and histidine. Clones also exhibited beta-galactosidase activity in both qualitative and quantitative assays. These results suggest that CP42 protein contains an amino acid motif able to activate transcription of His3 and lacZ reporter genes in Saccharomyces cerevisiae. Several deletions of the CP42 gene were cloned into the pGBT9 vector to locate the region involved in this activation. CP42 constructions lacking 12 residues from the C-terminal region and another one with 267 residues deleted from the N-terminus are still able to activate transcription of reporter genes. However, transcription activation was not observed with construction p9CP42deltaC57, which does not contain the last 57 amino acid residues. These results demonstrate that a transcription activation domain is present at the C-terminus of CP42 between residues 267 and 374.

Highlights

  • Andean potato mottle virus (APMoV) is a plant virus endemic in South America [1] and a member of the Comovirus genus and Comoviridae family, of which cowpea mosaic virus (CPMV) is the type member [2]

  • Clones exhibited ß-galactosidase activity in both qualitative and quantitative assays. These results suggest that CP42 protein contains an amino acid motif able to activate transcription of His3 and lacZ reporter genes in Saccharomyces cerevisiae

  • These results demonstrate that a transcription activation domain is present at the C-terminus of CP42 between residues 267 and 374

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Summary

Introduction

Andean potato mottle virus (APMoV) is a plant virus endemic in South America [1] and a member of the Comovirus genus and Comoviridae family, of which cowpea mosaic virus (CPMV) is the type member [2]. CP42 constructions lacking 12 residues from the C-terminal region and another one with 267 residues deleted from the N-terminus are still able to activate transcription of reporter genes. The results of transcriptional activation, obtained with the CP42 construct in the yeast system, will permit further experiments in order to determine a functional map of CP42 transactivation domains.

Results
Conclusion
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