首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Effect of dexamethasone on detection of herpes simplex virus in clinical specimens by conventional cell culture and rapid 24-well plate centrifugation.
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Effect of dexamethasone on detection of herpes simplex virus in clinical specimens by conventional cell culture and rapid 24-well plate centrifugation.

机译:地塞米松对常规细胞培养和24孔板快速离心检测临床标本中单纯疱疹病毒的影响。

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摘要

During a 4-month period, two methods for rapid detection of herpes simplex virus (HSV) were examined: (i) pretreatment of A549 cells with dexamethasone for conventional tissue culture (277 specimens) and (ii) 24-well plate centrifugation using A549 cells with and without dexamethasone pretreatment and staining with serotype-specific monoclonal antibodies (Syva Co., Palo Alto, Calif.) after incubation for 16 to 18 h (153 specimens). By conventional tube cell culture, both with and without dexamethasone, HSV was identified in 88 of 277 (32%) specimens. Significantly more specimens were positive for HSV at 24 h (46 versus 27 specimens) and at 48 h (a total of 72 versus 59 specimens) (P less than 0.0001) in dexamethasone-treated A549 cells. Of the 153 specimens tested by conventional culture and 24-well plate centrifugation, HSV was detected in 44 (29%) by conventional culture, and by 24-well plate centrifugation with and without dexamethasone, HSV was detected in 32 (21%) and 30 (20%) specimens, respectively. The sensitivity, specificity, and positive and negative predictive values of 24-well plate centrifugation with A549 cells for detection of HSV were 73 (71% without dexamethasone), 100, 100, and 90%, respectively. In conventional tube cell culture, pretreatment of A549 cells with dexamethasone results in more rapid detection of HSV. Centrifugal inoculation of dexamethasone-treated and untreated A549 cells in 24-well plates and staining with monoclonal antibodies after incubation for 16 to 18 h is an insensitive means to detect HSV in clinical specimens and should not replace conventional tube cell culture.
机译:在4个月的时间内,研究了两种快速检测单纯疱疹病毒(HSV)的方法:(i)用地塞米松预处理A549细胞用于常规组织培养(277个标本)和(ii)使用A549进行24孔板离心培养16至18小时(153个标本)后,对有或没有地塞米松预处理的细胞进行血清处理,并用血清型特异性单克隆抗体(Syva Co.,Palo Alto,CA)染色。通过常规的管细胞培养,无论是否使用地塞米松,在277个样本中有88个(32%)鉴定出HSV。在地塞米松处理的A549细胞中,在24小时(46比27个样本)和48小时(总共72比59个样本)的HSV阳性样本更多(P小于0.0001)。在常规培养和24孔板离心测试的153个标本中,常规培养检出HSV的有44个(29%),在有和没有地塞米松的情况下通过24孔板离心检测到的HSV的32例(21%)和分别有30个(20%)标本。用A549细胞进行24孔板离心检测HSV的敏感性,特异性以及阳性和阴性预测值分别为73(无地塞米松的71%),100、100和90%。在常规的管细胞培养中,用地塞米松预处理A549细胞可更快速地检测HSV。在24孔板中离心接种地塞米松处理的和未处理的A549细胞,并在孵育16至18 h后用单克隆抗体染色是检测临床标本中HSV的一种不灵敏的方法,不应替代常规的管细胞培养。

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