Real-time quantitative PCR for human herpesvirus 6 DNA

被引:108
作者
Locatelli, G
Santoro, F
Veglia, F
Gobbi, A
Lusso, P
Malnati, MS
机构
[1] Ist Sci San Raffaele, DIBIT, Unit Human Virol, I-20132 Milan, Italy
[2] Ist Sci San Raffaele, DIBIT, Biostat Unit, I-20132 Milan, Italy
[3] Univ Bologna, Dept Clin & Expt Med, I-40138 Bologna, Italy
关键词
D O I
10.1128/JCM.38.11.4042-4048.2000
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The diagnosis of human herpesvirus 6 (HHV-6) infection represents a complex issue because the most widely used diagnostic tools, such as immunoglobulin G antibody titer determination and qualitative DNA PCR with blood cells, are unable to distinguish between latent (clinically silent) and active (often clinically relevant) infection. We have developed a new, highly sensitive, quantitative PCR assay for the accurate measurement of HHV-6 DNA in tissue-derived cell suspensions and body fluids. The test uses a 5' nuclease, fluorogenic assay combined with real-time detection of PCR amplification products with the ABI PRISM 7700 sequence detector system. The sensitivity of this method is equal to the sensitivity of a nested PCR protocol (lower detection limit, I viral genome equivalent/test) for both the A and the B HHV-6 subgroups and shows a wider dynamic range of detection (from 1 to 10(6) viral genome equivalents/test) and a higher degree of accuracy, repeatability, and reproducibility compared to those of a standard quantitative-competitive PCR assay developed with the same reference DNA molecule. The novel technique is versatile, showing the same sensitivity and dynamic range with viral DNA extracted from different fluids (i.e., culture medium or plasma) or from tissue-derived cell suspensions, Furthermore, by virtue of its high-throughput format, this method is well suited for large epidemiological surveys.
引用
收藏
页码:4042 / 4048
页数:7
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