A Cosmid System for the Analysis of Lytic Replication of Epstein–Barr Virus

The resulting two-dimensional gel electrophoresis pattern (Fig. ), has reduced horizontal streaking and greater spot resolution compared to the gel pattern from acetone:methanol precipitation (Fig. ). Tri-n-butylphosphate, a lipophilic solvent, is thought to extract lipids by forming micelles (8) an

The 895-8 isolate of the Epstein-Barr virus (EBV) has been described as a non-lytic transforming virus. We have performed experiments in order to determine if the B95-8 EBV is capable of super-infecting and replicating in EBV-genomepositive non-producer lymphoblastoid cells. Using concentrates of 89

## Abstract Epstein‐Barr virus (EBV) latent and replicative gene transcription was analyzed in peripheral blood B‐lymphocytes from astronauts who flew on short‐duration (∼11 days) Shuttle missions and long‐duration (∼180 days) International Space Station (ISS) missions. Latent, immediate‐early, and

Epstein-Barr virus (EBV), provides unique advantages to understand origins of replication in higher eukaryotes. EBV establishes itself efficiently in infected B lymphocytes, where it exists as a 165 kb, circular chromosome which is duplicated once per cell cycle (Adams [1987] J Virol 61:1743-1746).