TY - JOUR
T1 - Re-examination by improved reverse transcriptase assay of DNA polymerase in platelets from myelodysplastic disease patients
AU - Yoshida, S.
AU - Yamada, H.
AU - Sakurai, T.
AU - Suzuki, M.
AU - Kojima, K.
PY - 1989
Y1 - 1989
N2 - A number of reports have suggested that platelets from polycythemia vera patients contain reverse transcriptase activity that might be correlated with C-type retrovirus-like particles. As described herein, we devised a new assay method for reverse transcriptase activity using MS-2 phage RNA hybridized with synthetic oligodeoxynucleotide (18-mer) as a template/primer. Using this new, sensitive assay method, we examined the platelet enzyme. By the conventional assay method using poly(rA)-oligo (dT), extracts of platelets showed a considerable amount of incorporation. However, by the new assay method using MS-2 RNA, no incorporation was observed. The poly(rA)-oligo(dT)-dependent activity was purified on Mono Q column, and it was shown that this activity coincided with that of DNA polymerase γ.
AB - A number of reports have suggested that platelets from polycythemia vera patients contain reverse transcriptase activity that might be correlated with C-type retrovirus-like particles. As described herein, we devised a new assay method for reverse transcriptase activity using MS-2 phage RNA hybridized with synthetic oligodeoxynucleotide (18-mer) as a template/primer. Using this new, sensitive assay method, we examined the platelet enzyme. By the conventional assay method using poly(rA)-oligo (dT), extracts of platelets showed a considerable amount of incorporation. However, by the new assay method using MS-2 RNA, no incorporation was observed. The poly(rA)-oligo(dT)-dependent activity was purified on Mono Q column, and it was shown that this activity coincided with that of DNA polymerase γ.
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M3 - Article
C2 - 2483974
AN - SCOPUS:0024440073
SN - 0158-5231
VL - 19
SP - 1133
EP - 1141
JO - Biochemistry International
JF - Biochemistry International
IS - 5
ER -