Diagnosis of Tubercular Lymphadenitis by PCR of Fine Needle Aspirates

M. Parvez, Mohiuddin, Z. Hassan, F. Ahmad, J. Haq
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引用次数: 5

Abstract

A definitive and accurate diagnosis of tubercular lymphadenitis is important for its proper management. Fine needle aspiration cytology (FNAC) is an easy procedure for collection of material for cytopathological and bacteriological examination. But the detection rate of M. tuberculosis from the aspirated material is low with Ziehl-Neelson (Z-N) stain and even with culture. Polymerase chain reaction (PCR) is a rapid method for diagnosis of tuberculosis from various clinical samples. In the present study, PCR was employed for the detection of mycobacterial DNA sequences in fine needle aspirates of twenty cases of suspected tubercular lymphadenitis and compared with cytomorphological characteristics, Z-N stain and culture. Thermo stable multiplex PCR was used to detect Mycobacterium specific DNA. The rate of PCR positivity for mycobacterial DNA was 70% as compared to 50% and 60% by Z-N stain and culture respectively. Papanicolaou as well as Hematoxylin and Eosin (HE 6(2): 46-49
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细针穿刺PCR诊断结核性淋巴结炎
明确和准确的诊断结核性淋巴结炎对其适当的治疗是重要的。细针吸细胞学(FNAC)是收集细胞病理学和细菌学检查材料的一种简单方法。但Ziehl-Neelson (Z-N)染色法和培养法对抽吸物结核分枝杆菌的检出率较低。聚合酶链反应(PCR)是一种快速诊断结核病的方法。本研究采用PCR方法对20例疑似结核性淋巴结炎细针抽吸液中的分枝杆菌DNA序列进行检测,并与细胞形态学特征、Z-N染色及培养进行比较。采用热稳定多重PCR检测分枝杆菌特异性DNA。分枝杆菌DNA PCR阳性率为70%,而Z-N染色法和培养法分别为50%和60%。Papanicolaou以及苏木精和伊红(HE 6(2): 46-49)
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