TY - JOUR
T1 - SV40 recombinants carrying rabbit β-globin gene coding sequences
AU - Hamer, Dean H.
AU - Smith, Kirby D.
AU - Boyer, Samuel H.
AU - Leder, Philip
N1 - Funding Information:
We thank Tom Maniatis for pflG2. George Khoury for assisting us with the in vitro transcription experiments, Jim Alwine for helping us with the RNA transfer experiments and David Rodbard for statistical analysis of the radioimmunoassay data. We are grateful to Terri Broderick for her expert assistance in the preparation of this manuscript. K.D.S. was supported by grants from the NIH and the NSF.
PY - 1979/7
Y1 - 1979/7
N2 - We have constructed and propagated two SV40 recombinants in which different portions of the viral late gene region are replaced by a rabbit β-globin coding sequence derived from a cloned cDNA (Maniatis et al., 1976). One of these recombinants, which retains the promoter, leader and intervening sequences for a viral late mRNA, directs the synthesis of a stable SV40-globin hybrid transcript. Using a sensitive radioimmunoassay, we have shown that this globin RNA is translated in infected monkey cells. A second recombinant, which retains the late region promoter but lacks the RNA splicing region, produces neither a stable globin transcript nor any detectable β-globin. These experiments indicate that some sequence within a 500 bp SV40 segment, presumably the splicing region, is required for the accumulation of stable mRNA. They also demonstrate how hybrid transducing viruses can be used both to characterize viral regulatory sequences and to produce new gene products in cultured cells.
AB - We have constructed and propagated two SV40 recombinants in which different portions of the viral late gene region are replaced by a rabbit β-globin coding sequence derived from a cloned cDNA (Maniatis et al., 1976). One of these recombinants, which retains the promoter, leader and intervening sequences for a viral late mRNA, directs the synthesis of a stable SV40-globin hybrid transcript. Using a sensitive radioimmunoassay, we have shown that this globin RNA is translated in infected monkey cells. A second recombinant, which retains the late region promoter but lacks the RNA splicing region, produces neither a stable globin transcript nor any detectable β-globin. These experiments indicate that some sequence within a 500 bp SV40 segment, presumably the splicing region, is required for the accumulation of stable mRNA. They also demonstrate how hybrid transducing viruses can be used both to characterize viral regulatory sequences and to produce new gene products in cultured cells.
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U2 - 10.1016/0092-8674(79)90279-4
DO - 10.1016/0092-8674(79)90279-4
M3 - Article
C2 - 225043
AN - SCOPUS:0018645296
SN - 0092-8674
VL - 17
SP - 725
EP - 735
JO - Cell
JF - Cell
IS - 3
ER -