TOP10 Electrocomp™ 试剂盒
TOP10 Electrocomp™ 试剂盒
Invitrogen™

TOP10 Electrocomp™ 试剂盒

TOP10 大肠杆菌的转化效率为 1 × 1010 cfu/µg 超螺旋 DNA,适用于高效克隆和质粒增殖。其可稳定复制高拷贝数质粒。TOP10了解更多信息
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货号数量
C664555 x 100μL
C6641110 x 100μL
货号 C66455
价格(CNY)
2,446.00
Each
添加至购物车
数量:
5 x 100μL
价格(CNY)
2,446.00
Each
添加至购物车
TOP10 大肠杆菌的转化效率为 1 × 1010 cfu/µg 超螺旋 DNA,适用于高效克隆和质粒增殖。其可稳定复制高拷贝数质粒。

TOP10 细胞的基因型与 DH10B™株相似,具有以下特点:

hsdR 用于通过 PCR 扩增高效转化未甲基化 DNA
mcrA 用于通过基因组制备高效转化甲基化
lacZΔM15 用于蓝/白斑筛选重组克隆
• 由于无需进行核酸内切酶 I 的非特异性酶切,endA1 用于在下游应用中获得更清洁的 DNA 制备物和更好的结果
recA1 用于降低克隆 DNA 中的非特异性重组

One Shot™ TOP10 试剂盒提供了化学感受态或电转感受态大肠杆菌,适用于您特定的转化需求。TOP10 大肠杆菌还提供了高通量 MultiShot™ 规格。

注:此试剂盒含有足够用于 12 x 40 µL 反应或 25 x 20 µL 反应的电转感受态细胞。有关反应规模建议,请参见产品手册。

基因型:
F-mcrA Δ(mrr-hsdRMS-mcrBC) φ80lacZΔM15 ΔlacX74 recA1 araD139 Δ(ara-leu)7697 galU galK rpsL endA1 nupG
仅供科研使用。不可用于诊断程序。
规格
耐抗生素细菌Yes (Streptomycin)
蓝色/白色筛查
是否可克隆甲基化 DNA
克隆不稳定 DNA不适合克隆不稳定DNA
是否含 F' 附加体缺乏 F’附加体
高通量能力不兼容高通量应用(手动)
提高质粒质量
质粒可用于 > 20 kb 质粒
制备无甲基化 DNA不适合制备未甲基化DNA
产品线DH10B,Electrocomp™
产品类型电转化仪试剂盒
数量5 x 100μL
减少克隆重组现象
运输条件Dry Ice
T1 噬菌体 - 抗性 (tonA)
转化效率级别高效率 (> 10^9 cfu⁄µg)
产品规格One Shot
种属大肠杆菌
Unit SizeEach
内容与储存
• 5 x 100μL TOP10 Electrocomp E. coli
• 50 μL pUC19 vector (10 pg/μL)
Store at –80°C.

• S.O.C. Medium (15 mL)
Store at room temperature.

常见问题解答 (FAQ)

TOP10细胞与TOP10F’细胞的区别是什么?

TOP10与TOP10F’细胞的区别仅在于后者包含F’游离体因而带有四环素抗性基因,而且能够从带有f1复制起点的载体菌株中分离单链DNA。F’ 游离体同时还带有lacIq抑制子,因此可用IPTG诱导trc、ta、和lac启动子的表达。TOP10F’细胞需要IPTG诱导进行蓝白斑筛选。

我正在尝试克隆一个毒性可能非常大的插入片段。我使用过DH5α和TOP10细胞进行转化但是没有在平板上得到克隆。你们能为我提供一些建议吗?

如果插入片段对于宿主细胞有潜在毒性,您可以尝试以下建议:

•转化TOP10或DH5α细胞后,在25-30摄氏度而不是在37摄氏度下孵育。这会降低生长速度并能提高克隆具有潜在毒性的插入片段的几率。
•尝试使用TOP10F’细胞进行转化,但是不在培养板中加入IPTG。这些细胞带lacIq阻抑物抑制从lac启动子起始表达,因此能克隆毒性基因。请注意,没有加入IPTG时不能进行蓝白斑筛选。
•尝试使用Stbl2细胞进行转化。

What is the difference between TOP10 and TOP10F' cells?

The only difference between TOP10 and TOP10F' cells is that the latter contain the F' episome that carries the tetracycline resistance gene and allows isolation of single-stranded DNA from vectors that have an f1 origin of replication. The F' episome also carries the lacIq repressor for inducible expression from trc, tac, and lac promoters using IPTG. TOP10F' cells require IPTG induction for blue/white screening.

I am trying to clone an insert that is supposedly pretty toxic. I used DH5? and TOP10 cells for the transformation and got no colonies on the plate. Do you have any suggestions for me?

If the insert is potentially toxic to the host cells, here are some suggestions that you can try:

- After transforming TOP10 or DH5? cells, incubate at 25-30°C instead of 37°C. This will slow down the growth and will increase the chances of cloning a potentially toxic insert.
- Try using TOP10F' cells for the transformation, but do not add IPTG to the plates. These cells carry the lacIq repressor that represses expression from the lac promoter and so allows cloning of toxic genes. Keep in mind that in the absence of IPTG, blue-white screening cannot be performed.
- Try using Stbl2 cells for the transformation.

Can I directly clone, propagate and express in BL21 without using TOP10?

It is imperative that a cloning strain such as TOP10 be used for characterization of the plasmid, propagation, and maintenance. BL21 cells are wild-type for endA and recA, which could result in poor miniprep quality and a greater chance of plasmid rearrangements due to recombination. In addition, BL21 cells contain the T7 RNA polymerase gene which is expressed at low levels even in the absence of inducer. If the gene is toxic to E. coli, plasmid instability and/or cell death can result.

View all TOP10 Electrocomp™ 试剂盒 FAQs