One Shot™ OmniMAX™ 2 T1R chemisch kompetente E. coli
One Shot&trade; OmniMAX&trade; 2 T1<sup>R</sup> chemisch kompetente <i>E. coli</i>
Invitrogen™

One Shot™ OmniMAX™ 2 T1R chemisch kompetente E. coli

Der One Shot™ OmniMAX™ 2 T1R E. coli-Stamm ist eine verbesserte, chemisch kompetente Zelllinie, perfekt für den Einsatz bei allenWeitere Informationen
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KatalognummerMenge
C85400321 x 50 μl
Katalognummer C854003
Preis (EUR)
480,00
Special offer
Online exclusive
Endet: 21-Jul-2025
510,00
Ersparnis 30,00 (6%)
Each
Vorrätig
Zum Warenkorb hinzufügen
Menge:
21 x 50 μl
Recurring order eligible. Learn more »
Preis (EUR)
480,00
Special offer
Online exclusive
Endet: 21-Jul-2025
510,00
Ersparnis 30,00 (6%)
Each
Zum Warenkorb hinzufügen
Ask our AI about this Product
Der One Shot™ OmniMAX™ 2 T1R E. coli-Stamm ist eine verbesserte, chemisch kompetente Zelllinie, perfekt für den Einsatz bei allen Klonierungs-Anwendungen, einschließlich Gateway™ Technologie. OmniMAX™ 2 T1R-Zellen haben die höchste Transformationseffizienz aller chemisch kompetenten Zellen im One Shot™ Format mit > 5 x 109 Transformanden/µg pUC19. Sie bieten zudem effiziente Transformation bei stark methylierter DNA, da OmniMAX™ 2 T1R-Zellen keine E. coli K12-Einschränkungssysteme haben (mcrA Δ(mrr hsdRMS-mcrBC)). Darüber hinaus umfasst der Stamm den ton-Genotyp, der für Resistenz gegenüber T1- und T5-Phagen-Infektion sorgt. Dies schützt Ihre Proben und minimiert mögliche Ausfallzeiten durch Phagen-Kontamination in Ihrem Labor. Der äußerst vielseitige OmniMAX™ 2 T1R-Stamm bietet folgende Vorteile:

• Ideal für die Transformation bei Gateway™ und TOPO™ Reaktionen
• T1- und T5-Phagen-Resistenz (tonA)
• Aufbau repräsentativerer Genbibliotheken dank Beseitigung von mcrA, mcrBC, mrr und hsdRMS
• Blau-Weiß-Screening rekombinanter Klone (lacZΔM15)

Genotyp: F´ {proAB lacIq lacZΔM15 Tn10(TetR ) Δ(ccdAB)} mcrA Δ(mrr hsdRMS-mcrBC) Φ80(lacZ)ΔM15 Δ(lacZYA-argF)U169 endA1 recA1 supE44 thi-1 gyrA96 relA1 tonA panD
Nur für Forschungszwecke. Nicht zur Verwendung bei diagnostischen Verfahren.
Specifications
Bakterielle AntibiotikaresistenzYes (Tetracycline)
Blau-Weiß-ScreeningJa
Klonierung methylierter DNAJa
Klonierung instabiler DNANicht geeignet zum Klonen instabiler DNA
Enthält F'-EpisomEnthält F'-Episom
Hochdurchsatz-KompatibilitätNicht mit hohen Durchsatz kompatibel (manuell)
Verbessert die PlasmidqualitätJa
PlasmidKann für Plasmide >20 kb verwendet werden
Vorbereitung von nicht methylierter DNANicht geeignet für die Vorbereitung von nicht methylierter DNA
ProduktlinieOne Shot™
ProdukttypKompetente Zelle
Menge21 x 50 μl
Reduziert RekombinationJa
VersandbedingungTrockeneis
T1-Phage – resistent (TonA)Ja
TransformationsleistungsgradHoher Wirkungsgrad (> 10^9 cfu⁄µg)
FormatRörchen
SpeziesE. coli
Unit SizeEach
Inhalt und Lagerung
Enthält:
• One Shot™ OmniMAX™ 2 T1R E. coli: 21 Fläschchen, je 50 µl
• pUC19 DNA (10 pg/µl): 1 Fläschchen, 50 µl
• S.O.C.-Medium: 1 Flasche, 6 ml

Kompetente Zellen bei -80 °C lagern. Lagern Sie pUC19 DNA bei -20 °C. SOC-Medium bei +4 °C oder Raumtemperatur lagern.
Ready-to-use Bacterial Growth Media

Ready-to-use Bacterial Growth Media

See how these mediums can help with critical aspects of cloning!

Gibco LB Broth

Invitrogen S.O.C. Medium

Invitrogen One Shot LB Agar*

*Only available in North America and selected European countries

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Häufig gestellte Fragen (FAQ)

What strain should I use to transform my library?

OmniMAX 2 is the preferred strain for transforming libraries because of its high transformation efficiency and genomic cloning compatibility characteristics.

What advantages do your Stbl2 cells offer over other cloning strains?

There are other strains available that may function similarly to Stbl2 cells in stabilizing inserts or vectors with repeated DNA sequences. However, one advantage of Stbl2 cells over many similar strains is that they are sensitive to Kanamycin, so you can use Stbl2 to propagate plasmids containing a Kanamycin resistance marker. 

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.

Do any Invitrogen competent cells contain DMSO in the freezing medium?

Yes, several of our competent cells products are frozen with DMSO. The presence of DMSO (dimethylsulfoxide) will generally be indicated in the MSDS files if you have a question about a particular product, but here is a list of commonly used products that are known to have DMSO in the freezing buffer:

One Shot OmniMAX 2 T1 Phage Resistant Cells, Cat. No. C8540-03

One Shot INV?F' Chemically Competent Cells, Cat. No. C2020-03 and C2020-06

One Shot MAX Efficiency DH5?-T1 Chemically Competent Cells, Cat. No. 12297-016

MAX Efficiency DH5?-T1 Phage Resistant Cells, Cat. No. 12034-013

MAX Efficiency DH5? Chemically Competent Cells, Cat. No. 18258-012

Library Efficiency DH5? Chemically Competent Cells, Cat. No. 18263-012

MAX Efficiency DH5? F'IQ Cells, Cat. No. 18288-019

MAX Efficiency Stbl2Chemically Competent Cells, Cat. No. 10268-019

Does the methylation status of DNA affect its ability to be cloned?

Yes. Bacterial host cells will often degrade incoming DNA that has a methylation pattern that is "foreign" relative to that of the cell. Several host strains have been modified to accept mammalian methylation patterns. The modified markers include mcrA, mcrBC, and mrr. Also, endogenous (b-type) restriction endonucleases can be problematic. Modifications of the host to be rK- or rB- are necessary and include hsdR17(AK-, MK+), hsdR17(rK-, mK-), hsdS20(rB-, rB-) or hsdRMS. Strains with the hsdR17(rK-, mK+) mutation lack K-type restriction endonuclease, but contain K-type methylase. DNA prepared from hosts that are rK- mK- is unmethylated and will transform with lower efficiency in rK+ hosts.

TOP10, DH10B, and OmniMAX2-T1 cells contain the mcr, mrr, and hsdRMS mutations. Mach1 and standard DH5? strains only have the hsdR17(rK- mK+) mutation and are not recommended for cloning eukaryotic genomic DNA.

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Zertifikate

Chargen-Nr.Certificate TypeDateCatalog Number(s)
3104180Certificate of Analysis27. März 2025C854003
3033107Certificate of Analysis01. Nov. 2024C854003
2893783Certificate of Analysis19. Juni 2024C854003
2792140Certificate of Analysis04. Jan. 2024C854003
2723626Certificate of Analysis01. Dez. 2023C854003
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