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Basic flow of molecular diagnosis

2022-01-05 13:36:05
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The core technologies of most molecular diagnostic laboratories are focused on detecting specific, relatively short fragments of DNA or RNA. The technology can diagnose infectious diseases, identify specific genetic variants that affect drug metabolism, or detect genes associated with diseases, such as those associated with cancer. At the heart of these assays is the use of real-time quantitative polymerase chain reaction (PCR), transcription-regulated amplification (TMA), targeted amplification, and signal amplification, among other similar technologies. Sanger sequencing and analysis of DNA fragments or gels using capillary electrophoresis are key techniques in molecular diagnostic laboratories, but they often also include an amplification step in the detection process. In order to successfully apply assays that use DNA and RNA to diagnose disease, molecular diagnostic laboratories need to use well-defined workflows that result in consistent, valid results, and there are existing tools that help diagnostic laboratories achieve each workflow. Special tools for streamlining.

The basic flow of detection is as follows:

1. Sample collection and preparation. Genes for testing are extracted from the sample.

2. Amplification: Once the genetic material is isolated, it is immediately amplified to a detectable amount so that a diagnostic order can be made.

3. Detection: After getting enough target substance, the light sensor will read the signal corresponding to the target substance to be detected. Signals can be single or multiple, enabling the detection of multiple target species in a single reaction (eg, multi-channel detection).

4. Data analysis: analyze the signal read in the detection step. The results of the analysis are converted into information that laboratory personnel can interpret at any time, ultimately providing the clinician with a diagnosis.

Molecular diagnostic reagent raw materials


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