Fast Tagment DNA Library Prep Kit For MGI
Fast Tagment DNA Library Prep Kit For MGI is a rapid library preparation kit optimized exclusively for the MGI platform. Its core technology adopts a high-efficiency transposase, which innovatively integrates three independent steps of traditional library construction—DNA fragmentation, end repair and adapter ligation—into a single enzymatic "Tagmentation" reaction. This integrated design drastically reduces the requirement for the starting amount of DNA samples and significantly shortens the library construction time, greatly improving experimental efficiency and throughput. The kit features simple operation and broad compatibility, and is suitable for a variety of sample types including genomic DNA. While ensuring the generated libraries have high quality, high uniformity and an ideal fragment distribution, it can rapidly and economically convert samples into sequencing libraries suitable for the MGI platform. It is an ideal solution for achieving rapid, stable and low-cost high-throughput library construction in fields such as genomics, transcriptomics and metagenomics, and is particularly suitable for large-scale sample screening and rapid detection projects.
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- Product Information
- Product Manual
Fast Tagment DNA Library Prep Kit For MGI
1. Product Overview
Fast Tagment DNA Library Prep Kit is a tailor-made solution for the MGI high-throughput sequencing platform. The kit can efficiently convert DNA samples into dedicated libraries applicable to the MGI sequencing platform. It adopts transposase technology to integrate multiple tedious steps required in traditional methods, such as DNA fragmentation, end repair and adapter ligation, into a single enzymatic reaction process. This technological breakthrough not only greatly reduces the amount of starting DNA required, but also significantly shortens the time needed for library construction.
2. Applications
Fast Tagment DNA Library Prep Kit For MGI leverages its special transposition mechanism to simultaneously complete two steps—DNA fragmentation and adapter ligation—in a single reaction. This "one-step" tagmentation method greatly simplifies the experimental workflow, which not only saves operation time but also reduces experimental costs, making the library construction process more efficient.
Figure 1. Schematic diagram of second-generation sequencing library construction
References
[1] Li N, Jin K, Bai Y, Fu H, Liu L, Liu B. Tn5 Transposase Applied in Genomics Research. Int J Mol Sci. 2020 Nov 6;21(21):8329. doi: 10.3390/ijms21218329.
[2] Zhang H, Lu T, Liu S, Yang J, Sun G, Cheng T, Xu J, Chen F, Yen K. Comprehensive understanding of Tn5 insertion preference improves transcription regulatory element identification. NAR Genom Bioinform. 2021 Oct 27;3(4):lqab094. doi: 10.1093/nargab/lqab094.
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