T4 DNA Polymerase
T4 DNA Polymerase
Citations & References (5)
Invitrogen™

T4 DNA Polymerase

T4 DNAポリメラーゼは、3´-エキソデオキシリボヌクレアーゼ活性を有しますが、5´a3´エキソデオキシリボヌクレアーゼ活性を有しないDNAポリメラーゼです。T4DNAポリメラーゼの技術資料が用意されています。アプリケーション:置換合成による直線状二本鎖DNAの標識(1)。オリゴヌクレオチド誘導、部位特異的変異誘発詳細を見る
テクニカルサポートオーダーサポート
表示を変更buttonViewtableView
製品番号(カタログ番号)数量
1800501750 U
18005025250 U
製品番号(カタログ番号) 18005017
価格(JPY)
16,200
Each
お問い合わせください ›
数量:
50 U
T4 DNAポリメラーゼは、3´-エキソデオキシリボヌクレアーゼ活性を有しますが、5´a3´エキソデオキシリボヌクレアーゼ活性を有しないDNAポリメラーゼです。T4DNAポリメラーゼの技術資料が用意されています。

アプリケーション:置換合成による直線状二本鎖DNAの標識(1)。オリゴヌクレオチド誘導、部位特異的変異誘発(2)。二本鎖DNAの3´末端標識(3)。5´または3オーバーハングの両方を研磨して平滑末端を形成(4)。

由来:プラスミド上のT4 DNAポリメラーゼ遺伝子を発現している大腸菌から精製。

性能および品質試験:一本鎖および二本鎖エンドデオキシリボヌクレアーゼおよびホスファターゼアッセイ。エキソデオキシリボヌクレアーゼおよびポリメラーゼ活性を試験。

ユニットの定義:1ユニットは、テンプレート/プライマーとしてDNase IニックDNAを用い、37℃、30分間で10 nMolのデオキシリボヌクレオチドを酸不溶性画分へ取り込ませるものとする。

ユニット反応条件:50 mMグリシンNaOH(pH 8.8)、16.6 mM(NH42SO4、6 mM MgCl2、6.5 µM EDTA、10 mM 2-メルカプトエタノール、0.165 mg/ml BSA、1.6 mg/ml DNase Iニックサーモン精巣DNA、0.33 mM dCTP、0.33 mM dATP、0.33 mM dGTP、0.33 mM dTTP、76 nM [3H] dTTP、酵素0.1 ml中で、37℃、30分間インキュベーション
研究用にのみ使用できます。診断用には使用いただけません。
仕様
概要DNAポリメラーゼ
エキソヌクレアーゼ活性3' - 5'
ホットスタート不可
ポリメラーゼT4 DNAポリメラーゼ
数量50 U
出荷条件湿氷
形状液体
Unit SizeEach
組成および保存条件
T4 DNAポリメラーゼには、5X T4 DNAポリメラーゼバッファー1バイアル[165 mMトリス酢酸塩(pH 7.9)、330 mM酢酸ナトリウム、50 mM酢酸マグネシウム、5 mm DTT]が付属しています。-20℃で保存

よくあるご質問(FAQ)

What enzymes can I use to convert a molecule with a 5' or 3' overhang to a blunt molecule? What is the main difference between them?

T4 DNA polymerase and Klenow fragment of E.coli DNA polymerase can both convert overhangs to blunt molecules. The 3' - 5' exonuclease activity of the T4 DNA polymerase is much more efficient than Klenow.

Is there anything to prevent AmpliTaq Gold DNA polymerase from extending from the 3’ end of a TaqMan probe in a 5’ nuclease assay?

Yes. There is a phosphate group on the 3' end of all TaqMan probes that prevents such extension.

How does AmpliTaq Gold DNA Polymerase differ from AmpliTaq DNA Polymerase?

AmpliTaq Gold DNA Polymerase is a modified form of AmpliTaq DNA Polymerase that contains a proprietary chemical (or so-called hot start molecule) bound to the enzyme's active site. In order to activate the AmpliTaq Gold DNA Polymerase fully, we recommend an initial activation step of 95 degrees C for 10 min when using GeneAmp 10X PCR Buffer I and/or GeneAmp 10X PCR Buffer II and Mg in one of our thermal cyclers. When using GeneAmp 10X PCR Gold Buffer, activation time can be reduced to 5 minutes. Once activation is complete, you can proceed with your standard PCR cycling program (denaturing, annealing, extension, etc).

Does AmpliTaq Gold DNA Polymerase contain exonuclease (proofreading) activity?

No, AmpliTaq Gold DNA polymerase does not contain proofreading activity, however fidelity in PCR amplifications utilizing this enzyme may be improved. High fidelity can be achieved by: 1. Decreasing the final concentration of each nucleotide to 40-50 uM. 2. Using the lowest MgCl2 concentration possible. 3. Using less enzyme. 4. Decreasing extension times. 5. Using the highest annealing temperature possible. 6. Using as few cycles as possible.

Does the fidelity of AmpliTaq DNA Polymerase change in the presence of base analogs?

The fidelity of this PCR enzyme is affected in two ways. First, AmpliTaq DNA Polymerase typically binds to and incorporates base analogs less efficiently than conventional dNTPs, which means that polymerase activity is lower in reactions that contain base analogs. Second, the analog may pair with more than one conventional complementary template base, so the analog may be incorporated at an increased level compared to conventional dNTPs. For the best fidelity, we recommend that base analogs are included at low concentrations in the reaction.

View all T4 DNA Polymerase, 50 U FAQs

引用および参考文献 (5)

引用および参考文献
Abstract
Authors:
Journal:
PubMed ID:16195417
Role of the E1A Rb-binding domain in repression of the NF-kappa B-dependent defense against tumor necrosis factor-alpha.
Authors: Cook James L; Walker Thomas A; Worthen G Scott; Radke Jay R;
Journal:Proc Natl Acad Sci U S A
PubMed ID:12119420
'The adenoviral E1A oncogene sensitizes mammalian cells to tumor necrosis factor-alpha (TNF-alpha), in part by repressing the nuclear factor-kappa B (NF-kappa B)-dependent defense against this cytokine. Other E1A activities involve binding to either p300/cyclic AMP response element-binding protein (CBP) or retinoblastoma (Rb)-family proteins, but the roles of E1A interactions with ... More
Identification of a Novel Transcription Factor, GAGATA-binding Protein, Involved in Androgen-mediated Expression of Prostate-specific Antigen.
Authors:Wang C, Yeung F, Liu PC, Attar RM, Geng J, Chung LW, Gottardis M, Kao C,
Journal:J Biol Chem
PubMed ID:12782640
'Prostate-specific antigen (PSA) is the most valuable marker for the evaluation of prostate cancer progression. The expression of PSA is controlled by androgen receptor (AR) through its binding to androgen-response elements (AREs). Several AREs have been identified within the 5.8-kb PSA promoter. The main activity of this 5.8-kb PSA promoter ... More
Characterization of the SECIS binding protein 2 complex required for the co-translational insertion of selenocysteine in mammals.
Authors:Kinzy SA, Caban K, Copeland PR,
Journal:Nucleic Acids Res
PubMed ID:16155186
'Selenocysteine is incorporated into at least 25 human proteins by a complex mechanism that is a unique modification of canonical translation elongation. Selenocysteine incorporation requires the concerted action of a kink-turn structural RNA (SECIS) element in the 3'' untranslated region of each selenoprotein mRNA, a selenocysteine-specific translation elongation factor (eEFSec) ... More
A simple method using T4 DNA polymerase to clone polymerase chain reaction products.
Authors: Wang K; Koop B F; Hood L;
Journal:Biotechniques
PubMed ID:7980913
None