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弯曲杆菌属菌种的检测:基于培养法和聚合酶链反应法的比较

Detection of campylobacter species: a comparison of culture and polymerase chain reaction based methods.

作者信息

Kulkarni S P, Lever S, Logan J M J, Lawson A J, Stanley J, Shafi M S

机构信息

Public Health Laboratory, Central Middlesex Hospital, Acton Lane, Park Royal, London NW10 7NS, UK.

出版信息

J Clin Pathol. 2002 Oct;55(10):749-53. doi: 10.1136/jcp.55.10.749.

Abstract

AIMS

To investigate the optimal method for the detection of campylobacters from stool samples by comparing selective culture with membrane filtration and the polymerase chain reaction (PCR).

METHODS

Three hundred and forty three stool samples were investigated by each of the three methods mentioned above. Selective culture was performed with charcoal cefoperazone desoxycholate agar plates. Membrane filtration was performed using cellulose triacetate membranes with 0.45 micro m pores placed on blood agar plates. Enteropathogenic campylobacters were detected using a PCR identification algorithm, consisting of screening PCRs and species identification using a PCR enzyme linked immunosorbent assay (PCR-ELISA), both based on the 16S rRNA gene.

RESULTS

Of the 343 samples tested, 23 were positive by one or more method. Of these, 17 were positive by selective culture, 12 by membrane filtration, and 20 by the PCR identification algorithm. A total of 18 of 23 positives were identified as C jejuni and/or C coli by the PCR identification algorithm, compared with 14 identified to the genus level by selective culture, and 10 by membrane filtration. Among the remaining five positive samples, one C hyointestinalis was detected only by the PCR identification algorithm; one C upsaliensis was detected only by the PCR identification algorithm; one Campylobacter sp was detected by membrane filtration and selective culture and later identified as C concisus; one Campylobacter sp was detected by membrane filtration alone and later identified as Arcobacter sp; and one Campylobacter sp detected only by selective culture was lost to study and therefore not speciated. There was no significant difference between detection by selective culture and the other two methods. However, detection by PCR was significantly better than by membrane filtration (0.05 > p > 0.02).

CONCLUSION

The PCR identification algorithm can detect and identify Campylobacter spp to the species level and the result is obtained on the same day. However, PCR is expensive, labour intensive, and does not provide an isolate for further identification or typing. Selective culture is as good as the PCR identification algorithm for the detection of the two most common species, C jejuni and C coli, and it is cheap and practical. However, it does miss the less common species, results take 48 hours, and identification is only to the genus level. Membrane filtration showed a low sensitivity compared with the other methods and is not appropriate for the diagnostic laboratory, although it was the only method to detect the Arcobacter sp. The optimum method for the detection of campylobacters from stool samples in the diagnostic laboratory remains selective culture.

摘要

目的

通过比较选择性培养、膜过滤法和聚合酶链反应(PCR),研究从粪便样本中检测弯曲杆菌的最佳方法。

方法

采用上述三种方法对343份粪便样本进行检测。使用活性炭头孢哌酮脱氧胆酸盐琼脂平板进行选择性培养。使用孔径为0.45μm的三醋酸纤维素膜置于血琼脂平板上进行膜过滤。采用PCR鉴定算法检测肠道致病性弯曲杆菌,该算法包括基于16S rRNA基因的筛选PCR和使用PCR酶联免疫吸附测定(PCR-ELISA)进行菌种鉴定。

结果

在343份检测样本中,23份样本通过一种或多种方法检测为阳性。其中,17份通过选择性培养呈阳性,12份通过膜过滤呈阳性,20份通过PCR鉴定算法呈阳性。通过PCR鉴定算法,23份阳性样本中有18份被鉴定为空肠弯曲菌和/或结肠弯曲菌,相比之下,选择性培养鉴定到属水平的有14份,膜过滤法鉴定到属水平的有10份。在其余5份阳性样本中,仅通过PCR鉴定算法检测到1份猪肠弯曲菌;仅通过PCR鉴定算法检测到1份乌普萨拉弯曲菌;通过膜过滤法和选择性培养检测到1份弯曲菌属菌株,随后鉴定为简明弯曲菌;仅通过膜过滤法检测到1份弯曲菌属菌株,随后鉴定为嗜低温栖热菌属菌株;仅通过选择性培养检测到1份弯曲菌属菌株,但在研究过程中丢失,因此未进行菌种鉴定。选择性培养与其他两种方法之间的检测结果无显著差异。然而,PCR检测明显优于膜过滤法(0.05>p>0.02)。

结论

PCR鉴定算法能够将弯曲杆菌属检测并鉴定到菌种水平,且结果可在同一天获得。然而,PCR成本高、劳动强度大,且无法提供用于进一步鉴定或分型的分离株。对于检测空肠弯曲菌和结肠弯曲菌这两种最常见的菌种,选择性培养与PCR鉴定算法效果相当,且成本低、实用性强。然而,它确实会遗漏不太常见的菌种,结果需要48小时,且仅能鉴定到属水平。与其他方法相比,膜过滤法灵敏度较低,虽然它是检测嗜低温栖热菌属菌株的唯一方法,但不适用于诊断实验室。诊断实验室从粪便样本中检测弯曲杆菌的最佳方法仍是选择性培养。

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