- ¥267.80
- Thermo Scientific
- USA
- EP0041
- 2025年07月13日
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- 详细信息
- 文献和实验
- 技术资料
- 保存条件:
-20
- 保质期:
2年
- 英文名:
thermo
- 库存:
1000
- 供应商:
北诺生命科学
- 规格:
500 units
公司产品线包括:FastDigest & 常规限制性内切酶、修饰酶、PCR & RT-PCR产品、核酸和蛋白质Markers、分子生物学试剂盒(分子克隆、核酸纯化、标记、检测)、转染试剂、核苷酸等。
Unstained Protein MW Marker, 2 x 1 mL. 26610(SM0431) Pierce
Prestained Protein MW Marker, 500 uL. 26612(SM0441) Pierce
PageRuler Unstained Protein Ladder, 2 x 250 uL. 26614(SM0661) Pierce
PageRuler Prestained Protein Ladder, 2 x 250 uL. 26616(SM0671) Pierce
PageRuler Prestained Protein Ladder, 10 x 250 uL. 26617(SM0672) Pierce
PageRuler Plus Prestained Protein Ladder, 2 x 250 uL. 26619(SM1811) Pierce
PageRuler Plus Prestained Protein Ladder, 10 x 250 uL. 26620(SM1812) Pierce
Spectra Multicolor Broad Range Protein Ladder, 10 x 250 uL. 26623(SM1842) Pierce
Spectra Multicolor High Range Protein Ladder, 2 x 250 uL. 26625(SM1851) Pierce
Spectra Multicolor Low Range Protein Ladder, 250 uL. 26628(SM1861) Pierce
PageRuler Broad Range Unstained Protein Ladder, 26630(SM1881) Pierce
PageRuler Low Range Unstained Protein Ladder, 2 x 250 uL. 26632(SM1891) Pierce
Spectra Multicolor Broad Range Protein Ladder, 2 x 250 uL. 26634(SM1841) Pierce
10X Buffer Cfr9I B02 Fermentas
10X Buffer Cfr10I B04 Fermentas
10X Buffer EcoRI B12 Fermentas
10X Buffer Bsp143I B13 Fermentas
Bovine Serum Albumin B14 Fermentas
10X Taq Buffer with KCl and 15 mM MgCl2 B16 Fermentas
Dilution Buffer for Restriction Enzymes B19 Fermentas
10X Buffer Eco52I B22 Fermentas
10X Buffer SduI, Ppu21I B23 Fermentas
10X Buffer SdaI B24 Fermentas
10X Buffer Eam1105I B25 Fermentas
10X Buffer Ecl136II, PacI, SacI B26 Fermentas
10X Buffer AarI, AjiI, Bpu10I, ScaI, PasI B27 Fermentas
10X Buffer TaqI B28 Fermentas
10X Buffer KpnI B29 Fermentas
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文献和实验We report a simple homogeneous fluorescence assay for quantification of DNA polymerase function in high throughput. The fluorescence signal is generated by the DNA polymerase triggering opening of a molecular beacon extension of the template
The Polymerase Chain Reaction (PCR)
. Did He Really Invent PCR? • The basic principle of replicating a piece of DNA using two primers had already been described by Gobind Khorana in 1971:– Kleppe et al. (1971) J. Mol. Biol. 56, 341-346. • Progress was limited by primer synthesis and polymerase
能催化从四种5′-脱氧核苷三磷酸游离出焦磷酸而使DNA进行聚合反应的酶。EC2.7.7.7.。必须以DNA为模板,合成的DNA与模板具有互补的碱基排列(碱基互补性)。是与DNA复制和修复有关的重要的酶,虽可从许多组织分离出来,但对大肠杆菌的这种酶的研究较为先进。康伯格(A.Kornberg,1958)最初从大肠杆菌将此酶纯化,并弄清了其结构和特异性,但以后经过分子遗传学的研究,已明确了这种酶主要与DNA修复有关。因此重新进行与DNA复制有关酶的检索,发现两种新的酶。康伯格最初发现的酶称为
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