
Clone PERV-C (A3) env was isolated from the genomic DNA of domestic pig (Sus scrofa domesticus) in Korea to investigate the molecular properties of PERV-C. The nucleic acid homologies between the PERV-MSL (type C) reference and the PERV-C(A3) clone was 99% for env, but a single base pair deletion was found in the transmembrane (TM) region of the env open reading frame. To examine the functional characteristics of truncated PERV-C env, we constructed a replication-incompetent retroviral vector by replacing the env gene of the pCL-Eco retrovirus vector with PERV-C env. A retroviral vector bearing PERV-C/A chimeric envelopes was also created to complement the TM defect. Our results indicated that truncated PERV-C env was not infectious in human cells as expected. Interestingly, however, the vector with the PERV-C/A envelope was able to infect 293 cells. This observation suggests that recombination within PERV-C TM could render PERV-C infectious in humans. To further characterize PERV-C/A envelopes, we constructed an infectious molecular clone by using a PCR-based technique. This infectious molecular clone will be useful to examine more specific regions that are critical for human cell tropism.
Recombination, Genetic, Korea, Molecular Sequence Data, Sus scrofa, Cell Line, Retroviridae, Viral Envelope Proteins, Animals, Humans, Point Mutation, Amino Acid Sequence, Cloning, Molecular, Sequence Alignment, Disease Reservoirs, Retroviridae Infections
Recombination, Genetic, Korea, Molecular Sequence Data, Sus scrofa, Cell Line, Retroviridae, Viral Envelope Proteins, Animals, Humans, Point Mutation, Amino Acid Sequence, Cloning, Molecular, Sequence Alignment, Disease Reservoirs, Retroviridae Infections
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