One Shot™ ccdB Survival™ 2 T1^R Competent Cells

본 제품은 LMO 제품으로, 고객 분께서 LMO 신고 시스템을 통해 직접 수입 신고를 진행해주셔야 합니다. 자세히보기

One Shot™ <i>ccd</i>B Survival™ 2 T1<sup>R</sup> Competent Cells

Invitrogen™

One Shot™ ccdB Survival™ 2 T1^R Competent Cells

One Shot™ ccdB Survival™ 2 T1 Phage-Resistant (T1R ) chemically competent E. coli는 ccdB 유전자 함유 플라스미드의 증식에 적합하며 Gateway™자세히 알아보기

카탈로그 번호	수량
A10460	11 x 50 μL

카탈로그 번호 A10460

제품 가격(KRW)

254,000

キャンペーン価格

Ends: 31-Mar-2026

290,000

할인액 36,000 (12%)

카트에 추가하기

11 x 50 μL

제품 가격(KRW)

254,000

キャンペーン価格

Ends: 31-Mar-2026

290,000

할인액 36,000 (12%)

카트에 추가하기

One Shot™ ccdB Survival™ 2 T1 Phage-Resistant (T1R ) chemically competent E. coli는 ccdB 유전자 함유 플라스미드의 증식에 적합하며 Gateway™ Vector Conversion System, Gateway™ destination, donor, super-coiled entry vector와 함께 사용하도록 만들어졌습니다. 형질전환 효율: >1 x 10^9 transformants⁄μg DNA.ccdB 생존율™ 2 T1R E. coli은 TOP10 strain에서 유래하여 다음과 같은 특징을 갖습니다.
-ccdB 유전자 산물 저항성
-T1 및 T5 phage 저항성(tonA)
-깨끗한 DNA 조제, endonuclease I (endA1)에 의한 비특이적 섭취를 없애 다음 단계 분석에서 우수한 결과 제공
-cloned DNA (recA1)에서 비특이적 재결합이 줄어듬
유전자형:
F- mcrA Δ(mrr-hsdRMS-mcrBC) Φ80lacZΔM15 ΔlacX74 recA1 araΔ139 Δ(ara-leu)7697 galU galK rpsL (StrR) endA1 nupG fhuA::IS2

For Research Use Only. Not for use in diagnostic procedures.

항생제 내성 박테리아Yes (Streptomycin)

블루/화이트 스크리닝Yes (lacZΔM15)

메틸화 DNA 클로닝Yes (mcrA)

불안정 DNA 클로닝Not suitable for cloning unstable DNA

에프에피솜 포함No

고처리량 호환성Low

플라스미드 품질 개선Yes (endA1)

플라스미드ccdB vector propagation

비메틸화 DNA 준비No

제품라인One Shot

제품 유형Chemically Competent Cells

수량11 x 50 μL

재조합 감소Yes (recA1)

배송 조건Dry Ice

T1 Phage - 저항성(tonA)Yes

형질전환 효율 수준High Efficiency (>1 x 10⁹ cfu/μg)

형식Tube

종E. coli (K12)

Unit SizeEach

구성 및 보관

• One Shot ccdB Survival 2 T1R Competent Cells (11 x 50 μL)
Store Competent Cells at &ndash80°C.

• pUC19 DNA (50 μL at 10 pg/μL)
Store pUC19 DNA at –20°C.

• S.O.C. Medium (6 ml)
Store S.O.C. Medium at 4°C or room temperature.

자주 묻는 질문(FAQ)

I just found out that Library Efficiency DB3.1 and One Shot ccdB Survival T1R cells have been discontinued. Do you offer an alternative for propagating ccdB-containing plasmids?

We offer One Shot ccdB Survival 2 T1^R cells (Cat. No. A10460) for propagating ccdB-containing plasmids.

What kind of competent cells should I use to propagate Donor vectors and Destination vectors? What cells should I use after the BP or LR recombination reaction?

All Donor vectors and Destination vectors contain the ccdB cell death gene to reduce background of non-recombined BP/LR plasmids. Therefore, growing non-recombined vector requires special cells (One Shot ccdB Survival 2 T1R Competent Cells) which are resistant to the lethal effects of ccdB. On the other hand, general E. coli cloning strains including TOP10 or DH5a may be used for plating the BP or LR reaction, or for propagation and maintenance of recombined Gateway constructs.

I need a competent cell strain that is ccdB resistant. The Library Efficiency DB3.1 cells you offer have been discontinued, as well as the One Shot ccdB Survival T1R chemically competent cells. What do you recommend?

Please use our ccdB Survival 2 T1R competent cell strain.

How do you recommend that I prepare my DNA for successful electroporation of E. coli?

For best results, DNA used in electroporation must have a very low ionic strength and a high resistance. A high-salt DNA sample may be purified by either ethanol precipitation or dialysis.

The following suggested protocols are for ligation reactions of 20ul. The volumes may be adjusted to suit the amount being prepared.

Purifying DNA by Precipitation: Add 5 to 10 ug of tRNA to a 20ul ligation reaction. Adjust the solution to 2.5 M in ammonium acetate using a 7.5 M ammonium acetate stock solution. Mix well. Add two volumes of 100 % ethanol. Centrifuge at 12,000 x g for 15 min at 4C. Remove the supernatant with a micropipet. Wash the pellet with 60ul of 70% ethanol. Centrifuge at 12,000 x g for 15 min at room temperature. Remove the supernatant with a micropipet. Air dry the pellet. Resuspend the DNA in 0.5X TE buffer [5 mM Tris-HCl, 0.5 mM EDTA (pH 7.5)] to a concentration of 10 ng/ul of DNA. Use 1 ul per transformation of 20 ul of cell suspension.

Purifying DNA by Microdialysis: Float a Millipore filter, type VS 0.025 um, on a pool of 0.5X TE buffer (or 10% glycerol) in a small plastic container. Place 20ul of the DNA solution as a drop on top of the filter. Incubate at room temperature for several hours. Withdraw the DNA drop from the filter and place it in a polypropylene microcentrifuge tube. Use 1ul of this DNA for each electrotransformation reaction.

When should DMSO, formamide, glycerol and other cosolvents be used in PCR?

Cosolvents may be used when there is a failure of amplification, either because the template contains stable hairpin-loops or the region of amplification is GC-rich. Keep in mind that all of these cosolvents have the effect of lowering enzyme activity, which will decrease amplification yield. For more information see P Landre et al (1995). The use of co-solvents to enhance amplification by the polymerase chain reaction. In: PCR Strategies, edited by MA Innis, DH Gelfand, JJ Sninsky. Academic Press, San Diego, CA, pp. 3-16.

Additionally, when amplifying very long PCR fragments (greater than 5 kb) the use of cosolvents is often recommended to help compensate for the increased melting temperature of these fragments.

Find additional tips, troubleshooting help, and resources within our PCR and cDNA Synthesis Support Center.

One Shot™ ccdB Survival™ 2 T1R Competent Cells