2021
DOI: 10.1101/2021.11.29.470340
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Design of novel specific primers for helicobacter detection with diagnostic utility evaluation of different 16srRNA genus-specific primers: A comparative study

Abstract: Molecular diagnosis of helicobacters by PCR is simpler, more accurate, and feasible compared to other diagnostic methods. Validity and accuracy are highly dependent on the PCR primer design, diffusion time, and mutation rate of helicobacters. This study aimed to design 16srRNA -specific primers for Helicobacter spp. and H. pylori. Application of comparative statistical analysis of the diagnostic utility of the most available 16srRNA genus-specific primers. The new primers were designed using bioinformatics too… Show more

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Cited by 1 publication
(3 citation statements)
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“…Animal samples: 5 samples were collected from Gastric autopsies from Mongrel dogs at the Surgery Department, Faculty of Veterinary Medicine, Cairo University. The samples were collected in sterile cups with sterile saline and transmitted to the Microbiology department, Faculty of Veterinary Medicine, Cairo University (Abdelmalek, et al, 2021) Isolation of H.pylori: Sample processing: The gastric biopsies and autopsies were homogenized by an electric automated homogenizer till all tissue disappeared within the fluid. (Rabiea, et al, 2021).…”
Section: This Study Was Approved By the Research Ethicsmentioning
confidence: 99%
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“…Animal samples: 5 samples were collected from Gastric autopsies from Mongrel dogs at the Surgery Department, Faculty of Veterinary Medicine, Cairo University. The samples were collected in sterile cups with sterile saline and transmitted to the Microbiology department, Faculty of Veterinary Medicine, Cairo University (Abdelmalek, et al, 2021) Isolation of H.pylori: Sample processing: The gastric biopsies and autopsies were homogenized by an electric automated homogenizer till all tissue disappeared within the fluid. (Rabiea, et al, 2021).…”
Section: This Study Was Approved By the Research Ethicsmentioning
confidence: 99%
“…PCR:The PCR mixture included 1x master mix (amaROnePCR TM , Cat.No. SM213-0250, GeneDireX, Inc.), 0.25 µmol forward, and reverse primers (ConsH), Forward primer: 5' TCG CTA AGA GAT CAG CCT ATG TCC T 3', Reverse primer: 5' ATT CCA CCT ACC TCT CCC ACA CT 3'.To produce 435bp (Abdelmalek et al 2021), 10 ng DNA, and up to 20 µl nuclease-free water. The amplification cycle for ConsH was as follow: initial denaturation at 94°C/3 minutes, 30 cycles of the following temperatures: 94°C/30 sec, annealing at 60°C/1 minutes, and cyclic extension at 72°C/2 minutes, final extension at 72°C/5 minutes.…”
Section: Molecular Identificationmentioning
confidence: 99%
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