Amplification of a full-length Borna disease virus (BDV) cDNA from total RNA of cells persistently infected with BDV

被引:6
|
作者
Shoya, Y
Kobayashi, T
Koda, T
Lai, PK
Tanaka, H
Koyama, T
Ikuta, K
Kakinuma, M
Kishi, M
机构
[1] HOKKAIDO UNIV,INST IMMUNOL SCI,SECT BACTERIAL INFECT,SCH MED,KITA KU,SAPPORO,HOKKAIDO 060,JAPAN
[2] HOKKAIDO UNIV,DEPT PSYCHIAT,SCH MED,KITA KU,SAPPORO,HOKKAIDO 060,JAPAN
[3] SALEM TEIKYO UNIV,DEPT BIOSCI,SALEM,WV 26426
关键词
BDV; full-length BDV cDNA; RT-PCR; DNA; RATS; ORGANIZATION; REPLICATION; SEQUENCE; PCR;
D O I
10.1111/j.1348-0421.1997.tb01881.x
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
We have developed a novel reverse transcriptase-polymerase chain reaction (RT-PCR) to amplify the full-length 8.9 kilobase (kbp) cDNA of the Borna disease virus (BDV) RNA genome from the total cellular RP;A of MDCK cells persistently infected with BDV (MDCK/BDV). Antigenomic BDV cDNA was reverse transcribed using a 53-mer oligonucleotide primer, corresponding to the 5'-terminus of a putative 3'-leader sequence of the BDV RNA genome, for 2 hr at 42 C followed by 30 min at 55 C. PCR was performed in the presence of this 53-mer antigenomic primer and a 25-mer primer, corresponding to the 3'-terminus of the BDV antigenomic cDNA, by use of an rTth DNA polymerase with proof-reading activity. The amplified full-length BDV cDNA was detected in as little as 20 ng of total cellular RNA of MDCK/BDV. This RT-PCR method should be a useful technique to study the molecular quasispecies of BDV.
引用
收藏
页码:481 / 486
页数:6
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