学术探索
学术期刊
新闻热点
数据分析
智能评审

COMPARISON OF SENSITIVITY FOR HUMAN CYTOMEGALOVIRUS OF THE POLYMERASE CHAIN-REACTION, TRADITIONAL TUBE CULTURE AND SHELL VIAL ASSAY BY SEQUENTIAL DILUTIONS OF INFECTED CELL-LINES

被引:22
作者
SANDIN, RL [1 ]
RODRIGUEZ, ER [1 ]
ROSENBERG, E [1 ]
PORTERJORDAN, K [1 ]
CAPARAS, M [1 ]
NASIM, S [1 ]
ROCKIS, M [1 ]
KEISER, JF [1 ]
GARRETT, CT [1 ]
机构
[1] GEORGE WASHINGTON UNIV,MED CTR,DEPT PATHOL,WASHINGTON,DC 20037
来源
JOURNAL OF VIROLOGICAL METHODS | 1991年 / 32卷 / 2-3期
关键词
POLYMERASE CHAIN REACTION; HUMAN CYTOMEGALOVIRUS; SHELL VIAL ASSAY; TRADITIONAL TUBE CULTURE;
D O I
10.1016/0166-0934(91)90049-6
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Although traditional tube culture (TTC) is still considered by many as the 'gold standard' for the laboratory diagnosis of human cytomegalovirus (HCMV), the shell vial assay (SVA) offers greater speed of detection. This technique utilizes immunofluorescence (IF) to detect early or immediate early nuclear antigens (IEA). The detection capabilities of these two tests were compared with the polymerase chain reaction (PCR), a technique that amplifies enzymatically selected DNA target sequences. Serial dilutions of crude culture harvests from 2 HCMV strains, Towne and a clinical urine isolate, were made up to 1:1 000 000. Ten-mu-l aliquots of the original sample and each dilution were tested by PCR, TTC and SVA. For PCR, the nested-primer approach was used. Outer primers delimited a 721-bp sequence contained within the 2nd to 4th exons of the immediate-early protein. Inner nest primers delimited a 167-bp sequence in the third exon, detected by a P-32-labelled probe. The results show that: (1) control samples which contained all PCR reagents but no DNA were uniformly negative; (2) radiolabelled-probe detection (RPD) of PCR products is, on average, 100 x more sensitive than detection by ethidium bromide; (3) PCR is, on average, 100 x more sensitive than evaluation of cytopathic effect (CPE) in the TTC; (4) the predictive value of a negative SVA results is low compared to PCR.
引用
收藏
页码:181 / 191
页数:11
相关论文
共 27 条
[1]  
APPERLEY JF, 1988, BONE MARROW TRANSPL, V3, P253
[2]   COMPARISON OF A LATEX AGGLUTINATION-TEST WITH 5 OTHER METHODS FOR DETERMINING THE PRESENCE OF ANTIBODY AGAINST CYTOMEGALO-VIRUS [J].
BECKWITH, DG ;
HALSTEAD, DC ;
ALPAUGH, K ;
SCHWEDER, A ;
BLOUNTFRONEFIELD, DA ;
TOTH, K .
JOURNAL OF CLINICAL MICROBIOLOGY, 1985, 21 (03) :328-331
[3]   PRIMER-MEDIATED ENZYMATIC AMPLIFICATION OF CYTOMEGALO-VIRUS (CMV) DNA - APPLICATION TO THE EARLY DIAGNOSIS OF CMV INFECTION IN MARROW TRANSPLANT RECIPIENTS [J].
CASSOL, SA ;
POON, MC ;
PAL, R ;
NAYLOR, MJ ;
CULVERJAMES, J ;
BOWEN, TJ ;
RUSSELL, JA ;
KRAWETZ, SA ;
PON, RT ;
HOAR, DI .
JOURNAL OF CLINICAL INVESTIGATION, 1989, 83 (04) :1109-1115
[4]  
CHEHAB FF, 1989, MODERN PATHOL, V2, P75
[5]   ROLE OF DEFECTIVE CYTOMEGALOVIRUS PARTICLES IN INDUCTION OF HOST-CELL DNA-SYNTHESIS [J].
DEMARCHI, JM ;
KAPLAN, AS .
VIROLOGY, 1977, 82 (01) :93-99
[6]   DETECTION OF CYTOMEGALO-VIRUS IN URINE FROM NEWBORNS BY USING POLYMERASE CHAIN-REACTION DNA AMPLIFICATION [J].
DEMMLER, GJ ;
BUFFONE, GJ ;
SCHIMBOR, CM ;
MAY, RA .
JOURNAL OF INFECTIOUS DISEASES, 1988, 158 (06) :1177-1184
[7]   EFFECT OF AGE OF SHELL VIAL MONOLAYERS ON DETECTION OF CYTOMEGALO-VIRUS FROM URINE SPECIMENS [J].
FEDORKO, DP ;
ILSTRUP, DM ;
SMITH, TF .
JOURNAL OF CLINICAL MICROBIOLOGY, 1989, 27 (09) :2107-2109
[8]   RAPID DETECTION OF CYTOMEGALOVIRUS IN MRC-5-CELLS INOCULATED WITH URINE SPECIMENS BY USING LOW-SPEED CENTRIFUGATION AND MONOCLONAL-ANTIBODY TO AN EARLY ANTIGEN [J].
GLEAVES, CA ;
SMITH, TF ;
SHUSTER, EA ;
PEARSON, GR .
JOURNAL OF CLINICAL MICROBIOLOGY, 1984, 19 (06) :917-919
[9]   ENZYMATIC AMPLIFICATION OF HUMAN CYTOMEGALO-VIRUS SEQUENCES BY POLYMERASE CHAIN-REACTION [J].
HSIA, K ;
SPECTOR, DH ;
LAWRIE, J ;
SPECTOR, SA .
JOURNAL OF CLINICAL MICROBIOLOGY, 1989, 27 (08) :1802-1809
[10]   A NOVEL VIRUS-LIKE INFECTIOUS AGENT IN PATIENTS WITH AIDS [J].
LO, SC ;
SHIH, JW ;
YANG, NY ;
OU, CY ;
WANG, RY .
AMERICAN JOURNAL OF TROPICAL MEDICINE AND HYGIENE, 1989, 40 (02) :213-226
123