DEVELOPMENT OF A SUPERSENSITIVE POLYMERASE CHAIN-REACTION METHOD FOR HUMAN T-LYMPHOTROPIC VIRUS TYPE-II (HTLV-II) AND DETECTION OF HTLV-II PROVIRAL DNA FROM BLOOD-DONORS IN JAPAN

被引:8
作者
HAMAKADO, T
MATSUMOTO, T
KOYANAGI, Y
HAYASHI, K
FUKADA, K
KOUCHIYAMA, T
YOSHIDA, T
YAMAMOTO, N
机构
[1] TOKYO MED & DENT UNIV,SCH LOW TEMP ENGN PHYS,DEPT MICROBIOL,TOKYO 113,JAPAN
[2] FUJIREBIO INC,UBE RES LAB,UBE,YAMAGUCHI,JAPAN
[3] FUKUOKA RED CROSS BLOOD CTR,FUKUOKA,JAPAN
[4] YAMAGUCHI RED CROSS BLOOD CTR,YAMAGUCHI,JAPAN
关键词
HTLV-II; PCR; BLOOD DONOR;
D O I
10.1007/BF01703061
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
A supersensitive polymerase chain reaction procedure was developed to detect human T-lymphotropic virus type II (HTLV-II) proviral genome. Six primer pairs covering the various regions of HTLV-II were compared and selected on the basis of specificity and sensitivity. Among them, one primer pair of the pol region of HTLV-II (II pol) was able to amplify and detect even 0.1 fg of the cloned plasmid HTLV-II DNA (seven copies) by regular ethidium bromide staining on polyacrylamide gel. By using this procedure, we screened 189 HTLV-I seropositive blood donors from Yamaguchi and Fukuoka Red Cross Blood Centers, Japan. There were four positive samples detectable with the HTLV-II-specific pol primer pair, as well as with the HTLV-I tax primer pair. The amplified DNAs of two specimens were cloned and sequenced. The sequences of the HTLV-I tax region from both specimens were identical to that of HTLV-I. On the other hand, those of the HTLV-II pol region were identical to that of HTLV-II, except for one base substitution in a clone from one subject. These results indicate that dual infection of HTLV-I and HTLV-II in the same persons occurs among Japanese blood donors.
引用
收藏
页码:119 / 129
页数:11
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