Rapid Detection of Rifampicin- and Isoniazid-Resistant Mycobacterium tuberculosis Using Real-Time PCR

Rapid Detection of Rifampicin- and Isoniazid-Resistant Mycobacterium tuberculosis Using Real-Time PCR


چاپ صفحه		 پژوهان
صفحه نخست سامانه		 چکیده مقاله
چکیده مقاله		 نویسندگان
نویسندگان		 دانلود مقاله
دانلود مقاله		 دانشگاه علوم پزشکی تبریز
دانشگاه علوم پزشکی تبریز

نویسندگان: خلیل انصارین , لیلا صاحبی , صفر فرج نیا , مجید خلیلی

کلمات کلیدی: MULTIPLE RIFAMPIN; DRUG-RESISTANCE; MUTATIONS; ASSAY; STRAINS; RELAPSE; IRAN

نشریه: 22262 , 10 , 9 , 2016

اطلاعات کلی مقاله
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نویسنده ثبت کننده مقاله خلیل انصارین
مرحله جاری مقاله تایید نهایی
دانشکده/مرکز مربوطه مرکز تحقیقات سل و بیماری های ریوی
کد مقاله 64555
عنوان فارسی مقاله Rapid Detection of Rifampicin- and Isoniazid-Resistant Mycobacterium tuberculosis Using Real-Time PCR
عنوان لاتین مقاله Rapid Detection of Rifampicin- and Isoniazid-Resistant Mycobacterium tuberculosis Using Real-Time PCR
ناشر 6
آیا مقاله از طرح تحقیقاتی و یا منتورشیپ استخراج شده است؟ بلی
عنوان نشریه (خارج از لیست فوق)
نوع مقاله Original Article
نحوه ایندکس شدن مقاله ایندکس شده سطح یک – ISI - Web of Science
آدرس لینک مقاله/ همایش در شبکه اینترنت

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Background: Accurate and rapid detection of drug-resistant Mycobacterium tuberculosis is fundamental for the successful treatment of tuberculosis (TB). Objectives: The aim of this study was to determine the frequency of common mutations leading to isoniazid (INH) and rifampicin (RMP) resistance. Patients and Methods: In a cross-sectional study carried out in 2014, 90 patients with M. tuberculosis from five border provinces of Iran were selected. After a full clinical history and physical evaluation, real-time polymerase chain reaction (PCR) technique was performed for the detection of mutations in the patients' katG and rpoB genes. The results were compared with results of a standard proportion method as well as a multiplex allele-specific PCR (MAS-PCR). Results: A total of 23 mutations were found in isolates among which, codon katG 315, rpoB P1 (511-519 sequence) and rpoB P2 (524-533 sequence) were responsible for seven, nine and seven cases, respectively. The mean(standard deviation (SD)) of melting temperature (Tm) in katG 315 codon, rpoB P1 and P2 sequences in susceptible and mutant isolates was as follows: katG 85.4 degrees C (0.18) and 87.54 degrees C (0.62); rpo B P1 84.6 degrees C (0.61) and 82.9 degrees C (0.38); rpo B P2 83.4 degrees C (0.18) and 85.3 degrees C (0.19), respectively. In comparison to the standard proportion test, the sensitivity of real-time PCR in detecting INH- and RMP-resistant mutations was 75% and 83.3%, respectively. In comparison to the MAS-PCRtest, 100% of katG 315 mutations and 80% of rpoB mutations were determined. Overall, 10% of the patients were diagnosed with a recurrence of TB. Age and previous history of TB treatment increased mutation odds in rpoB sequences (P = 0.046, P = 0.036, respectively). Conclusions: Detection of drug resistance associated with mutations through real-time PCR by melting analysis technique showed a high differentiating power. This technique had high concordance with the standard proportion test and MAS-PCR results.

نویسندگان
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نویسنده نفر چندم مقاله
خلیل انصاریندوم
لیلا صاحبیاول
صفر فرج نیاچهارم
مجید خلیلیششم

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