Electrophoretic Mobility-Shift Assay (EMSA) Kit, with SYBR™ Green & SYPRO™ Ruby EMSA stains

Citations & References (14)

Invitrogen™

Electrophoretic Mobility-Shift Assay (EMSA) Kit, with SYBR™ Green & SYPRO™ Ruby EMSA stains

この蛍光ベースの電気泳動移動度シフトアッセイ（EMSA）キットは、核酸とタンパク質の両方を同一のゲルで検出するための迅速かつ簡単で定量的な方法を提供します。このキットは、RNAまたはDNA検出用のSYBR™ グリーンEMSA核酸ゲル染色と、タンパク質検出用のSYPRO™ ルビーEMSAタンパク質ゲル染色の2種類の蛍光色素を使用して検出します詳細を見る

製品番号（カタログ番号）	数量
E33075	1 kit

製品番号（カタログ番号） E33075

価格（JPY）

103,600

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1 kit

一括またはカスタム形式をリクエストする

この蛍光ベースの 電気泳動移動度シフトアッセイ（EMSA）キットは、核酸とタンパク質の両方を同一のゲルで検出するための迅速かつ簡単で定量的な方法を提供します。このキットは、RNAまたはDNA検出用のSYBR™ グリーンEMSA核酸ゲル染色と、タンパク質検出用のSYPRO™ ルビーEMSAタンパク質ゲル染色の2種類の蛍光色素を使用して検出します。核酸およびタンパク質は電気泳動後にゲル内で連続的に染色されるため、標識がアッセイ中のタンパク質結合を阻害する可能性はありません。核酸の染色には約20分、その後のタンパク質染色には約4時間かかります。

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。

アッセイEMSA（電気泳動移動シフトアッセイ）

検出法蛍光

製品ラインSYBR、SYPRO

製品タイプ電気泳動モビリティシフトアッセイ（EMSA）キット

数量1 kit

出荷条件室温

Unit SizeEach

組成および保存条件

フリーザー（-5～-30度）に保存し、遮光してください。

よくあるご質問（FAQ）

What is a "supershift"?

A supershift assay is a method for positively identifying a protein:DNA interaction on an EMSA. An antibody (typically 1 µg) is added to the binding reaction. During electrophoresis, the antibody:protein:DNA complex migrates slowly, causing a “supershift” compared to the “shift” caused by a protein:DNA complex. Not all antibodies will cause a supershift. Some antibodies do not bind to proteins once they are bound to DNA. Some antibodies can prevent protein:DNA interactions but can still be used to confirm the identity of a protein that causes a shift in the absence of the antibody.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

What is an electrophoretic mobility shift assay (EMSA)?

EMSAs (also called gel shifts, band shifts, gel retardation assays, or mobility assays) have been used extensively for studying protein-DNA interactions. Because protein-DNA complexes migrate more slowly through a native polyacrylamide or agarose gel than DNA alone, individual protein-DNA complexes can be visualized as discrete bands within the gel using chemiluminescence or radioisotopic detection.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

What is a shift assay? What is a supershift assay?

A shift assay is a DNA-binding assay using nondenaturing PAGE. It provides a simple, rapid, and extremely sensitive method for detecting sequence-specific DNA-binding proteins. Proteins bind specifically to an end-labeled DNA fragment corresponding to the individual protein-DNA complexes. You can use the assay to test binding of purified proteins or of uncharacterized factors in crude extracts. This assay also permits quantitative determination of the affinity, abundance, association rate constants, dissociation rate constants, and binding specificity of DNA-binding proteins.

A supershift assay is a variation of the mobility shift DNA-binding assay that uses antibodies to identify proteins present in the protein-DNA complex.Addition of a specific antibody to a binding reaction can have one of several effects. If the protein recognized by the antibody is not involved in complex formation, addition of the antibody should have no effect. If the protein that forms the complex is recognized by the antibody, the antibody can either block complex formation or it can form an antibody-protein-DNA ternary complex and thereby specifically result in a further reduction in the mobility of the protein-DNA complex (a supershift). Results may be different depending upon whether the antibody is added before or after the protein binds DNA (particularly if there are epitopes on the DNA binding surface of the protein).

Find additional tips, troubleshooting help, and resources within our Nucleic Acid Purification and Analysis Support Center.

What is the composition of the 5X Binding Buffer included within Electrophoretic Mobility-Shift Assay (EMSA) Kit, with SYBR Green & SYPRO Ruby EMSA stains (Cat. No. E33075)?

Here is the composition of the 5X Binding Buffer:

- 50 mM Tris HCl, pH 7.4
- 750 mM KCl
- 0.5 mM DTT
- 0.5 mM EDTA

Note: This buffer is optimized for lac repressor binding to lac operator. It may not be optimal for other protein-nucleic acid interactions.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

引用および参考文献 (14)

引用および参考文献

Abstract

Regulation of Mn-superoxide dismutase activity and neuroprotection by STAT3 in mice after cerebral ischemia.

Authors:Jung JE, Kim GS, Narasimhan P, Song YS, Chan PH,

Journal:J Neurosci

PubMed ID:19474327

'Cerebral ischemia and reperfusion increase superoxide anions (O(2)(*-)) in brain mitochondria. Manganese superoxide dismutase (Mn-SOD; SOD2), a primary mitochondrial antioxidant enzyme, scavenges superoxide radicals and its overexpression provides neuroprotection. However, the regulatory mechanism of Mn-SOD expression during cerebral ischemia and reperfusion is still unclear. In this study, we identified the ... More

The N-terminus of the human RecQL4 helicase is a homeodomain-like DNA interaction motif.

Authors:Ohlenschläger O, Kuhnert A, Schneider A, Haumann S, Bellstedt P, Keller H, Saluz HP, Hortschansky P, Hänel F, Grosse F, Görlach M, Pospiech H,

Journal:Nucleic Acids Res

PubMed ID:22730300

'The RecQL4 helicase is involved in the maintenance of genome integrity and DNA replication. Mutations in the human RecQL4 gene cause the Rothmund-Thomson, RAPADILINO and Baller-Gerold syndromes. Mouse models and experiments in human and Xenopus have proven the N-terminal part of RecQL4 to be vital for cell growth. We have ... More

nalD encodes a second repressor of the mexAB-oprM multidrug efflux operon of Pseudomonas aeruginosa.

Authors:Morita Y, Cao L, Gould VC, Avison MB, Poole K,

Journal:J Bacteriol

PubMed ID:17028276

The Pseudomonas aeruginosa nalD gene encodes a TetR family repressor with homology to the SmeT and TtgR repressors of the smeDEF and ttgABC multidrug efflux systems of Stenotrophomonas maltophilia and Pseudomonas putida, respectively. A sequence upstream of mexAB-oprM and overlapping a second promoter for this efflux system was very similar ... More

Functional characterization of the NfxB repressor of the mexCD-oprJ multidrug efflux operon of Pseudomonas aeruginosa.

Authors:Purssell A, Poole K,

Journal:

PubMed ID:23924707

The mexCD-oprJ multidrug efflux operon of Pseudomonas aeruginosa is regulated by the NfxB repressor. Two forms of NfxB have been reported [Shiba et al. (1995). J Bacteriol 177, 5872) although mutagenesis studies here confirm that the larger protein (199 amino acids, 22.4 kDa) is the functional repressor. NfxB binds upstream ... More

Identifying cis-regulatory changes involved in the evolution of aerobic fermentation in yeasts.

Authors:Lin Z, Wang TY, Tsai BS, Wu FT, Yu FJ, Tseng YJ, Sung HM, Li WH,

Journal:Genome Biol Evol

PubMed ID:23650209

Gene regulation change has long been recognized as an important mechanism for phenotypic evolution. We used the evolution of yeast aerobic fermentation as a model to explore how gene regulation has evolved and how this process has contributed to phenotypic evolution and adaptation. Most eukaryotes fully oxidize glucose to CO2 ... More

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