فن حدیث میں مولانا عبد الرحمن مبارک پوری کی خدمات کا جائزہ

Sūnan-ul-Tirmizi is an encyclopedia of Ahādith-ul-Ahkām. Imam Tirmizi is the Mohadith who divided hadiths into Sahih and Zaeef for the first time. He accepts or rejects a hadith on the base of Taāmul-e-Ummah. He is only the Mohadith who established the terminology of “Filbāb” in which he gives the words of hadith from a Sahabi and mentions the names of all other sahabies who are rawi of the same hadith. There are many sharh of Tirmizi written by Muhadiseen. Among them Tuhfat ul Ahwazi is famously written by Molana Abdul Rahman Mubarakpuri. He explores the terminologies of Sonan-e-Tirmizi. He discussed uloom ul hadith, books of hadith, Shoroh-ul-hadith, Asma-ul-rejal and ilm ul ansab etc. He mentions tafsiri aqwal, fiqhi problems and usool-e-hadith. He also solved the Tasaholat-e-Tirmizi in validity (sihat) and unvalidity (zouf). He is the first mohadith who tried to find the words of hadith from other sahabies whose names are given in “Filbab”. He did it but could not find the words of 87 ahadith for which he used the term “Lam aqif alaih” and 417 ahadith for which he used the term “Le Yonzar man akhraja haza ul hadith”. This thing makes it distinct from other shoroh of Sūnan-e-Tirmizi. He depends on the usool-e-hadith of forefather Muhadiseen and he did not establish his own usool hadith.

Diagnostic Accuracy of a Commercial Cross Priming Amplification Diagnostic Kit in Smear Negative Sputum

Background: The diagnosis of smear negative tuberculosis remains a major obstacle to global control of tuberculosis (TB), especially in resource limited settings. Several nucleic acid based diagnostic tests have been developed to improve diagnosis. The polymerase chain reaction has been the benchmark for nucleic acid amplification; many novel alternatives have been developed for the amplification and detection of nucleic acid sequences. Objective: The study aimed to determine the diagnostic accuracy of Cross Priming Amplification technology using the Ustar TB Isothermal Amplification Diagnostic (IAD) Kit (Ustar Biotech, Hangzhou, China) in smear negative sputum. Methods: 159 unconcentrated sputum samples negative by direct Ziehl-Neelsen staining referred to the National Central Reference Lab in Nairobi were subjected to both the Ustar TB Isothermal Amplification Diagnostic Kit and culture. The reference standard was TB culture. Results: When tested on Ziehl-Neelsen negative smear sputum, the IAD assay was found to have a sensitivity of 75% (60-86%; 95% CI); Positive Predictive Value (PPV) of 84% (71-94%; 95% CI) and Diagnostic Odds Ratio of 42.18 (15.65-113.69; 95% CI). The specificity of the assay was 94% (87-97%; 95% CI). Conclusion: The assay demonstrated good sensitivity and moderate specificity in detecting mycobacterium tuberculosis in smear negative specimen, the requirements for a clean room for the DNA extraction procedure, a high speed centrifuge and biological safety chamber may limit the applicability of this technique in resource limited settings.