小鼠 Cot-1 DNA

引用和文献 (2)

Invitrogen™

小鼠 Cot-1 DNA

小鼠 Cot-1 DNA™ 是小鼠 DNA，大多数为50至 300 bp，且富含重复 DNA 序列，如 B1了解更多信息

货号	数量
18440016 又称 18440-016	500 μg

货号 18440016

又称 18440-016

价格（CNY)

4,849.00

添加至购物车

500 μg

价格（CNY)

4,849.00

添加至购物车

小鼠 Cot-1 DNA™ 是小鼠 DNA，大多数为50至 300 bp，且富含重复 DNA 序列，如 B1、B2 和 L1 家族成员。小鼠 Cot-1 DNA™ 通常用于封闭微阵列筛选中的非特异性杂交。它还可用于抑制啮齿动物重复 DNA 序列的杂交（当使用原位杂交或 Southern 印迹法对啮齿动物克隆进行映射时），识别源自小鼠-仓鼠杂交细胞的体细胞杂交文库筛选中的小鼠克隆 (1-3)。提供的量足以进行5至10次 Southern 或500次原位杂交。

性能和质量检测：通过琼脂糖凝胶电泳验证纯度和 DNA 大小。采用分光光度法，通过在 50 mM NaOH 中以 1:100 的比例稀释小鼠 Cot-1 DNA™ 并使用转换因子 0.033 µg/µL/A 260 验证浓度。其他用于测定浓度的方法可能会产生不同的结果。

仅供科研使用。不可用于诊断程序。

适用于（应用）阻断非特异性杂交

产品线Cot-1 DNA

产品类型小鼠 DNA

数量500 μg

试剂类型Cot-1 DNA

运输条件经批准可置于湿冰或干冰上运输

Unit SizeEach

内容与储存

小鼠 Cot-1 DNA™ 以 1 mg/mL 溶液形式提供，溶剂为 10 mM Tris-HCl（pH 值 7.4）、1 mM EDTA。在 -20°C 下储存。

常见问题解答 (FAQ)

How much COT-1 DNA should I use to suppress repetitive sequences during hybridization?

For Southern blot hybridizations, add 50 µg of COT-1 DNA (at 10 µg/µL) to 50 µL of 20X SSC, 25 µL distilled water and 20 µL of a solution containing 0.1 M NaCl, 0.1 M Tris-HCl (pH 7.4). 0.01 M EDTA, and 1% SDS to the probe for each 25 to 500 ng of probe. For in situ hybridizations, combine genomic probe with the proper amount of COT-1 DNA such that the final concentration of COT-1 DNA is 0.3 µg/µL for cosmid, plasmid, and lambda probes; or, at 1 µg/µL for Alu PCR probes. Ethanol precipitate and resuspend in a half-volume of 100% formamide. Add a half-volume of 20% dextran sulfate in 2X SSC (prewarmed to 75 degrees C) and mix well. Denature mix by heating to 75 degrees C for 5 min. Incubate at 37 degrees C for 5 to 15 min.

How can I label COT-1 DNA?

Probes can be labeled with 32P by random primer or nick translation procedures using the Random Primers DNA Labeling System (Cat. No.18187-013) or Nick Translation System (Cat. No. 18160-010). Biotinylated COT-1 DNA can be prepared by nick translation with the BioNick Labeling System (Cat. No. 18247-015) or by the BioPrime DNA Labeling System (Cat. No. 18094-011). Improved results can be obtained when the COT-1 DNA is first ligated to itself to provide an optimum template.

引用和文献 (2)

引用和文献

Abstract

A whole-genome mouse BAC microarray with 1-Mb resolution for analysis of DNA copy number changes by array comparative genomic hybridization.

Authors:Chung YJ, Jonkers J, Kitson H, Fiegler H, Humphray S, Scott C, Hunt S, Yu Y, Nishijima I, Velds A, Holstege H, Carter N, Bradley A,

Journal:Genome Res

PubMed ID:14707179

'Microarray-based comparative genomic hybridization (CGH) has become a powerful method for the genome-wide detection of chromosomal imbalances. Although BAC microarrays have been used for mouse CGH studies, the resolving power of these analyses was limited because high-density whole-genome mouse BAC microarrays were not available. We therefore developed a mouse BAC ... More

Rapid physical mapping of cloned DNA on banded mouse chromosomes by fluorescence in situ hybridization.

Authors:Boyle A L; Feltquite D M; Dracopoli N C; Housman D E; Ward D C;

Journal:Genomics

PubMed ID:1733847

Physical mapping of DNA clones by nonisotopic in situ hybridization has greatly facilitated the human genome mapping effort. Here we combine a variety of in situ hybridization techniques that make the physical mapping of DNA clones to mouse chromosomes much easier. Hybridization of probes containing the mouse long interspersed repetitive ... More