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TransStart^? FastPfu Fly DNA Polymerase

FastPfu Fly 快速高保真DNA 聚合酶

目錄號(hào)	規(guī)格	單價(jià)
AP231-21	250 units	770
AP231-22	500 units	1390
AP231-23	6×500 units	7060

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產(chǎn)品詳情介紹

TransStart^?FastPfu Fly DNA Polymerase是用于快速PCR的熱啟動(dòng)超高保真DNA聚合酶。該酶與TransStart^? FastPfu DNA Polymerase相比，擴(kuò)增速度更快（≤5 kb基因可實(shí)現(xiàn)12 kb/min的極速擴(kuò)增，＞5 kb基因可達(dá)到6 kb/min高速擴(kuò)增），擴(kuò)增效率更高，產(chǎn)量更高，保真性更高，靈敏度更高。2×TransStart^? FastPfu Fly Reaction Mix中已含有dNTPs，DNA擴(kuò)增時(shí)，只需加入模板、引物、水和TransStart^? FastPfu Fly DNA Polymerase，使Reaction Mix的濃度為1×即可進(jìn)行反應(yīng)。擴(kuò)增產(chǎn)物為平末端，可直接克隆于pEASY^?-Blunt系列載體中。

? 保真性是EasyTaq^? DNA Polymerase的108倍。

? 擴(kuò)增產(chǎn)物為平末端，可直接克隆于pEASY^?-Blunt系列載體中。

? 基因組DNA片段的擴(kuò)增（≤15 kb）。

? Plasmid DNA片段擴(kuò)增（≤ 20 kb）。

產(chǎn)品組成

實(shí)驗(yàn)數(shù)據(jù)

使用TransGen、Company TA及Company N產(chǎn)品，分別以人gDNA為模板，進(jìn)行不同基因的PCR擴(kuò)增，1.0%瓊脂糖凝膠電泳分析擴(kuò)增效果。

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References

1.Xu Y, Zhu T F. Mirror-image T7 transcription of chirally inverted ribosomal and functional RNAs[J]. Science, 2022.(IF 63.71)

2.Niu X, Tang W, Liu Y, et al. Prime editor-based high-throughput screening reveals functional synonymous mutations in human cells[J]. Nature Biotechnology, 2025.(IF 41.70)

3.Niu L, Shen W, Shi Z, et al. Three-dimensional folding dynamics of the Xenopus tropicalis genome[J]. Nature Genetics, 2021.(IF 38.33)

4.Duan Z, Liang Y, Sun J, et al. An engineered Cas12i nuclease that is an efficient genome editing tool in animals and plants[J]. The Innovation, 2024.(IF 33.20)

5.Huang M E, Qin Y, Shang Y, et al. C-to-G editing generates double-strand breaks causing deletion, transversion and translocation[J]. Nature Cell Biology, 2024.(IF 21.30)

6.Wang D, Yan F, Wu P, et al. Global profiling of regulatory elements in the histone benzoylation pathway[J]. Nature Communications, 2022.(IF 17.69)

7.Jin S, Fei H, Zhu Z, et al. Rationally designed APOBEC3B cytosine base editors with improved specificity[J]. Molecular cell, 2020.(IF 15.58)

8.Zhang A, Shan T, Sun Y, et al. Directed evolution rice genes with randomly multiplexed sgRNAs assembly of base editors[J]. Plant Biotechnology Journal, 2023.(IF 13.80)

9.Zhang Y F, Yun J H, Zhang G Y, et al. Efficient biosynthesis of 3-hydroxypropionic acid from glucose through multidimensional engineering of Escherichia coli[J]. Bioresource Technology, 2023.(IF 11.40)

10.Wang J L, Wang M, Zhang L, et al. WAV E3 ubiquitin ligases mediate degradation of IAA32/34 in the TMK1-mediated auxin signaling pathway during apical hook development[J]. Proceedings of the National Academy of Sciences, 2024.(IF 11.10)

11.Wang Y, Li S Y, Wang Y Z, et al. ZmASY1 interacts with ZmPRD3 and is crucial for meiotic double‐strand break formation in maize[J]. New Phytologist, 2023.(IF 9.40)

12.Li J, Bai Y, Liu Y, et al. Transcriptome-based chemical screens identify CDK8 as a common barrier in multiple cell reprogramming systems[J]. Cell Reports, 2023.(IF 8.80)

13.Jiang L, Yao B, Zhang X, et al. Salicylic acid inhibits rice endocytic protein trafficking mediated by OsPIN3t and clathrin to affect root growth[J]. The Plant Journal, 2023.(IF 7.20)

14.Tan Y, Yan X, Sun J, et al. Genome‐wide enhancer identification by massively parallel reporter assay in Arabidopsis[J]. The Plant Journal, 2023.(IF 7.20)

15.Chen J, Hu X, Shi T, et al. Metabolite‐based genome‐wide association study enables dissection of the flavonoid decoration pathway of wheat kernels[J]. Plant Biotechnology Journal, 2020.(IF 6.84)

16.Zhu J, Miao Q, Tang J, et al. Nucleolin mediates the internalization of rabbit hemorrhagic disease virus through clathrin-dependent endocytosis[J]. PLoS pathogens, 2018.(IF 6.16)

17.Chen J, Wang H, Yang X, et al. Consumption of miRNA-mediated insect-resistant transgenic rice pollen does not harm Apis mellifera adults[J]. Journal of Agricultural and Food Chemistry, 2021.(IF 5.30)

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