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PCR System Display
The real-time Quantitative PCR System offers several advantages over traditional PCR methods. Some of the key advantages include:
1. Quantification of target DNA: The real-time qPCR system allows for the accurate quantification of target DNA or RNA molecules. It measures the fluorescence signal generated during each amplification cycle, allowing for the determination of the initial amount of target DNA or RNA present in the sample. This quantitative aspect is particularly useful in gene expression analysis, viral load quantification, and copy number variation analysis.
2. High sensitivity and specificity: The real-time qPCR system is highly sensitive, capable of detecting very low amounts of target DNA or RNA. This sensitivity allows for the detection of rare genetic variants, low viral loads, or small changes in gene expression levels. Additionally, the system offers high specificity by using specific primers or probes that can target unique regions of the genome, minimizing non-specific amplification and decreasing the chances of false-positive results.
3. Rapid and real-time monitoring: The real-time qPCR system provides real-time monitoring of the amplification process, allowing researchers to track the progress of the reaction as it occurs. It provides information about the number of cycles required to reach a certain threshold level of amplification (threshold cycle or Ct value). This real-time monitoring allows for the detection of PCR inhibition, troubleshooting, and optimization of reaction conditions.
4. Wide dynamic range: The dynamic range of the real-time qPCR system refers to the ability to accurately quantify target DNA or RNA over a wide range of concentrations. This dynamic range can span several orders of magnitude, enabling the detection and quantification of both high and low abundance targets within a single assay.
5. Multiplexing capability: Real-time qPCR allows for the simultaneous detection and quantification of multiple targets in a single reaction. By using different fluorophores or probes with specific emission spectra, several targets or genes can be amplified and quantified in a single well. This saves time and reagents, making high-throughput analysis more efficient and cost-effective.
6. Minimal post-PCR handling: Real-time qPCR eliminates the need for post-PCR handling, such as gel electrophoresis, as the detection and quantification are performed during the PCR process itself. This reduces the chance of contamination and saves valuable time and effort.
7. Standardized and reproducible results: Real-time Quantitative PCR Machine provides more standardized and reproducible results compared to traditional endpoint PCR methods. The use of fluorescent dyes or probes and the integration of software for data analysis reduce user-dependent variability and allow for more accurate and consistent results.
8. Compatibility with other molecular techniques: Real-time qPCR can be easily integrated with other molecular biology techniques, such as reverse transcription (RT-qPCR) for gene expression analysis or next-generation sequencing (NGS) for validation and quantification of targets.
These advantages make real-time qPCR a powerful and versatile technique used in various fields of research, diagnostic testing, and clinical applications.
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April 23, 2024
April 23, 2024
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Mr. Mr. Leon Wen
Telefonnummer:0086-025-57561788
Fax:
Mobiltelefon:+8619871200893
E-Mail-Adresse:wenjiajun@superyears.com
Firmenadresse:Nanjing, Jiangsu
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Privacy statement: Your privacy is very important to Us. Our company promises not to disclose your personal information to any external company with out your explicit permission.