Zitierungen und Referenzen (20)

Invitrogen™

Taq DNA Polymerase, native

Name: Taq DNA Polymerase, native
SKU: 18038018
Price: 84.25 EUR

Taq DNA-Polymerase ist ein thermostabiles Enzym, das DNA aus einsträngigen Templates in Gegenwart von dNTPs und einem Primer synthetisiert. DasWeitere Informationen

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Katalognummer	Menge
18038018	100 Einheiten
18038042	500 Einheiten
18038067	3 x 500 Einheiten
18038240	5000 Einheiten

4 Optionen

Katalognummer 18038018

Preis (EUR)

84,25

Each

Menge:

100 Einheiten

Großbestellung oder individuelle Größe anfordern

Preis (EUR)

84,25

Each

Taq DNA-Polymerase ist ein thermostabiles Enzym, das DNA aus einsträngigen Templates in Gegenwart von dNTPs und einem Primer synthetisiert. Das Enzym besteht aus einem einzelnen Polypeptid mit einer Molekülmasse von 94 kDa. Es besitzt eine 5´→3´-DNA-Polymeraseaktivität und eine 5´→3´-Exonukleaseaktivität (siehe Abbildung). Vorteile der Taq DNA-Polymerase:

Sie haben die Wahl zwischen rekombinantem oder nativem Enzym

Amplifikation von bis zu 5 kb großen PCR-Produkten

Für PCR lizenziertes und zugelassenes Enzym

Anwendungen
Amplifikation von DNA aus komplexen genomischen, viralen oder Plasmid-Templates, RT-PCR, ssDNA-Sequenzierung Zyklus-Sequenzierung

Quelle
Natives Enzym, aufgereinigt aus Thermus aquaticus-YT1.

Definition einer Einheit
Eine Einheit Taq DNA-Polymerase ist die Enzymmenge, die benötigt wird, um in 30 Minuten bei 74 °C 10 nmol Desoxyribonukleotid in die DNA zu integrieren.

Nur für Forschungszwecke. Nicht für die Diagnostik bestimmt.

Specifications

Exonukleaseaktivität5' – 3'

Wiedergabetreue (vs. Taq)1X

FormatEigenständiges Enzym

Hot-StartNein

Anzahl Reaktionen100 Reaktionen

Überhang3'-A

PolymeraseTaq DNA-Polymerase

ProdukttypDNA-Polymerase

Menge100 Einheiten

ReaktionsformatSeparate Komponenten

VersandbedingungZugelassen für den Versand auf Nass- oder Trockeneis

Größe (Endprodukt)5 kb oder weniger

AusgangsmaterialDNA

Konzentration5 U/μl

Zur Verwendung mit (Anwendung)Standard-PCR

GC-Rich PCR PerformanceNiedrig

PCR-MethodeqPCR, Standard-PCR

ReaktionsgeschwindigkeitStandard

Unit SizeEach

Inhalt und Lagerung

Enthält:
• 20 µl Taq DNA-Polymerase (5 E/µl)
• 1,25 ml 10X PCR-Puffer (ohne Magnesium)
• 1 ml Magnesiumchlorid (50 mM)

Bei -20 °C in einem Gefriergerät ohne Abtauautomatik lagern. Bei ordnungsgemäßer Lagerung 6 Monate lang haltbar.

Häufig gestellte Fragen (FAQ)

My oligonucleotide does not appear to be the right length when I checked by gel electrophoresis. Why is this?

Oligos should be run on a polyacrylamide gel containing 7 M urea and loaded with a 50% formamide solution to avoid compressions and secondary structures. Oligos of the same length and different compositions can electrophorese differently. dC's migrate fastest, followed by dA's, dT's, and then dG's. Oligos containing N's tend to run as a blurry band and generally have a problem with secondary structure.

The primers I am using worked for PCR initially, but over time, have stopped working. What happened?

Primers should be aliquoted for single use before PCR set-up. Heat just the aliquoted primers to 94 degrees for 1 min. Quick chill the primer on ice before adding to the PCR reaction. Some primers may anneal to themselves or curl up on themselves.

I don't see a pellet in my oligo tube order. Should I ask for a replacement?

The drying method dries the primer in a thin layer along the sidewalls of the tube instead of the bottom, therefore a pellet is not always visible and should still be ready to use.

There is a ball-shaped pellet at the bottom of my oligo tube. What is this and can I still use my oligo?

If the oligo was overheated, it will appear as a “ball”-shaped pellet attached to the bottom of the tube. This should not affect the quality of the oligo, and the oligo should be readily soluble in water.

There is a green color in my lyophilized oligo. Can I still use it?

If an oligo appears green in color, this is most likely due to ink falling into the tube. The oligo should still be fully functional. The color can be removed by doing an ethanol precipitation.

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Zitierungen und Referenzen (20)

Zitierungen und Referenzen

Abstract

Sp3 Represses Gene Expression via the Titration of Promoter-specific Transcription Factors.

Authors: Kennett Sarah B; Moorefield K Scott; Horowitz Jonathan M;

Journal:J Biol Chem

PubMed ID:11773047

'We have determined previously that Sp3 encodes three distinct gene products as follows: a full-length protein (Sp3) that is an activator of transcription and two isoforms (M1 and M2) derived via internal translational initiation that function as transcriptional repressors. To identify amino acids and functions required for transcriptional repression, we ... More

Both DNA and histone fold sequences contribute to archaeal nucleosome stability.

Authors: Bailey Kathryn A; Marc Frederic; Sandman Kathleen; Reeve John N;

Journal:J Biol Chem

PubMed ID:11751933

'The roles and interdependence of DNA sequence and archaeal histone fold structure in determining archaeal nucleosome stability and positioning have been determined and quantitated. The presence of four tandem copies of TTTAAAGCCG in the polylinker region of pLITMUS28 resulted in a DNA molecule with increased affinity (DeltaDeltaG of approximately 700 ... More

Nuclear factor-kappa B directs carcinoembryonic antigen-related cellular adhesion molecule 1 receptor expression in Neisseria gonorrhoeae-infected epithelial cells.

Authors: Muenzner Petra; Billker Oliver; Meyer Thomas F; Naumann Michael;

Journal:J Biol Chem

PubMed ID:11751883

'The human-specific pathogen Neisseria gonorrhoeae expresses opacity-associated (Opa) protein adhesins that bind to various members of the carcinoembryonic antigen-related cellular adhesion molecule (CEACAM) family. In this study, we have analyzed the mechanism underlying N. gonorrhoeae-induced CEACAM up-regulation in epithelial cells. Epithelial cells represent the first barrier for the microbial pathogen. ... More

Methylation-mediated silencing of TMS1/ASC is accompanied by histone hypoacetylation and CpG island-localized changes in chromatin architecture.

Authors: Stimson Krista M; Vertino Paula M;

Journal:J Biol Chem

PubMed ID:11733524

'Aberrant methylation of CpG-dense islands in the promoter regions of genes is an acquired epigenetic alteration associated with the silencing of tumor suppressor genes in human cancers. In a screen for endogenous targets of methylation-mediated gene silencing, we identified a novel CpG island-associated gene, TMS1, which is aberrantly methylated and ... More

Functional coadaptation between cytochrome c and cytochrome c oxidase within allopatric populations of a marine copepod.

Authors: Rawson Paul D; Burton Ronald S;

Journal:Proc Natl Acad Sci U S A

PubMed ID:12271133

'Geographically isolated populations may accumulate alleles that function well on their own genetic backgrounds but poorly on the genetic backgrounds of other populations. Consequently, interpopulation hybridization may produce offspring of low fitness as a result of incompatibilities arising in allopatry. Genes participating in these epistatic incompatibility systems remain largely unknown. ... More

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