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在恰尔肯德邦西姆德加区不同村庄炭疽疫情爆发期间对循环菌株的分子确认

Molecular confirmation of the circulating during outbreak of anthrax in different villages of Simdega District, Jharkhand.

作者信息

Kumar Manoj, Seema Kumari, Prasad Amber, Sharma Ashok Kumar, Sherwal Banke Lal

机构信息

Department of Microbiology, RIMS, Ranchi, Jharkhand, India.

Rajiv Gandhi Super Speciality Hospital, New Delhi, India.

出版信息

Indian J Med Microbiol. 2019 Jan-Mar;37(1):116-119. doi: 10.4103/ijmm.IJMM_19_111.

Abstract

AIMS AND OBJECTIVES

Molecular confirmation of the circulating Bacillus anthracis during outbreak of anthrax in different villages of Simdega district, Jharkhand, India.

MATERIALS AND METHODS

Blood samples with swabs from skin lesions (eschar) were collected from the suspected cases of Anthrax from October 2014 to June 2016 from Simdega district, Jharkhand. All the swabs were inoculated on polymyxin lysozyme EDTA thallous acetate media, nutrient agar media as well as 5% sheep blood agar media. Gamma-phage lysis was done. DNA extraction was done using a QIAamp DNA Mini Kit (QIAGEN, Valencia, CA, USA) and subjected to polymerase chain reaction (PCR) using anthrax-specific primers.

RESULTS

On Gram and acid fast staining, purple rods and pink-coloured anthrax spores were detected. Capsular and M'Fadyean staining was done. Gamma-phage lysed B. anthracis culture. Of 39 suspected cases, 8 were culture and PCR positive and showed gamma-phage lysis. 3 deaths were reported.

DISCUSSION AND CONCLUSION

The conventional and real-time PCR methods are suitable for both the clinical and the epidemiological practice.

摘要

目的与目标

对印度贾坎德邦辛德加区不同村庄炭疽疫情期间循环的炭疽芽孢杆菌进行分子鉴定。

材料与方法

于2014年10月至2016年6月从贾坎德邦辛德加区疑似炭疽病例采集带有皮肤损伤(焦痂)拭子的血样。所有拭子接种于多粘菌素溶菌酶EDTA醋酸铊培养基、营养琼脂培养基以及5%绵羊血琼脂培养基上。进行γ噬菌体裂解试验。使用QIAamp DNA Mini试剂盒(美国加利福尼亚州瓦伦西亚的QIAGEN公司)进行DNA提取,并使用炭疽特异性引物进行聚合酶链反应(PCR)。

结果

革兰氏染色和抗酸染色检测到紫色杆菌和粉红色炭疽芽孢。进行荚膜染色和麦克法迪恩染色。γ噬菌体裂解炭疽芽孢杆菌培养物。39例疑似病例中,8例培养及PCR呈阳性并显示γ噬菌体裂解。报告了3例死亡病例。

讨论与结论

传统PCR方法和实时PCR方法适用于临床和流行病学实践。

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