Sexually transmitted disease assay kit MOLgen
DNA extractionTrichomonas vaginalisGardnerella vaginalis

Sexually transmitted disease assay kit - MOLgen  - ADALTIS - DNA extraction / Trichomonas vaginalis / Gardnerella vaginalis
Sexually transmitted disease assay kit - MOLgen  - ADALTIS - DNA extraction / Trichomonas vaginalis / Gardnerella vaginalis
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Characteristics

Applications
for sexually transmitted diseases, DNA extraction
Micro-organism
Gardnerella vaginalis, Trichomonas vaginalis
Sample type
clinical, urine, urogenital
Analysis mode
for real-time PCR, fluorescence

Description

“MOLgen DNA Trichomonas vaginalis / Gardnerella vaginalis S1 Kit” is an assay kit for the detection of Trichomonas vaginalis and Gardnerella vaginalisDNA by real-time PCR. Introduction “MOLgen DNA Trichomonas vaginalis / Gardnerella vaginalis S1 Kit”is intended for the detection of Trichomonas vaginalis and Gardnerella vaginalis DNA using the method of real-time polymerase chain reaction (PCR) with fluorescence detection of amplified product. DNA can be extracted from clinical specimens (urogenital and cervical swabs, semen, prostate fluid, urine) using “Molgen Universal Extraction Kit”. When using DNA extraction kits of other manufacturers it is highly recommended to use Internal Control sample (IC) manufactured by Adaltis. The results of PCR analysis are taken into account in complex diagnostics of disease. Set 1 is intended for use with block-type PCR cyclers: iQ iCycler, iQ5 iCycler (Bio-Rad, USA). The kit is compatible with other real-time PCR cyclers such as CFX96 (Bio-Rad, USA) and DT-96 (DNA-Technology, Russia). Set 1 contains reagents requiredfor 96 tests, including control samples. Principle Of Method Real-time PCR is based on the detection of the fluorescence produced by a reporter molecule, which increases as the reaction proceeds. Reporter molecule is a dual-labeled DNA-probe that specifically binds to the target region of pathogens DNA. Fluorescence signal increases due to the separation of fluorescence dye and quencher by Taq DNA-polymerase exonuclease activity during amplification. PCR consists of repeated cycles: temperature denaturation of DNA, primer annealing and complementary chain synthesis.

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