HA标签小鼠单克隆抗体(4F6),磁珠偶联

Name: HA标签小鼠单克隆抗体(4F6),磁珠偶联
Brand: Abbkine
SKU: ABT2044
Price: 2498 CNY
Availability: InStock

Magnetic Beads Conjugated Anti-HA Tag Mouse Monoclonal Antibody (4F6)

产品货号

ABT2044

产品特点：

磁珠表面共价偶联高亲和力小鼠抗HA单克隆抗体（4F6），1 ml磁珠可结合≥1 mg HA标签蛋白，富集效率高。

小鼠IgG1亚型，低非特异结合，适用于哺乳动物及细菌来源样本。

即用型液体形式，PBS缓冲液（pH 7.4，含0.02 % NaN₃）保存，4 °C可稳定一年，避免反复冻融。

冰袋运输，实验前无需额外活化或封闭，简化IP流程。

选择规格

1 mL

¥2498

现货（次日发货）

5 mL

¥12298

期货（3天内发货）

🎉 限时优惠

买2送1活动进行中！购买任意2个规格产品，免费赠送100μL装一支。

活动截止时间：2024年1月31日

产品概述

HA标签小鼠单克隆抗体（4F6），磁珠偶联是一种将小鼠源抗HA标签单克隆抗体（克隆号4F6）共价偶联于磁珠表面的即用型免疫沉淀工具，专为快速、高效地富集或纯化带HA标签的重组蛋白而设计。

Human influenza hemagglutinin (HA) 是一种位于流感病毒表面的糖蛋白，对病毒入侵宿主细胞至关重要。其98–106位氨基酸序列（YPYDVPDYA）被开发为通用表位标签（HA tag），已广泛应用于真核与原核表达系统。由于该标签体积小、免疫原性低，通常不会影响重组蛋白的生物活性或体内分布，因此成为研究蛋白–蛋白相互作用、信号转导及蛋白定位的理想标记。本抗体以合成HA多肽为免疫原，经亲和层析从小鼠腹水中纯化后，再与超顺磁磁珠共价偶联，可直接用于哺乳动物及细菌裂解液中HA标签蛋白的免疫沉淀（IP）实验。

应用领域

适用于免疫沉淀（IP）、Co-IP、pull-down等蛋白互作研究，以及HA标签重组蛋白的快速富集与纯化，广泛用于信号转导、蛋白复合体鉴定、药物靶点验证等基础与转化研究。

产品参数

中文名称	HA标签小鼠单克隆抗体(4F6),磁珠偶联
英文名称	Magnetic Beads Conjugated Anti-HA Tag Mouse Monoclonal Antibody (4F6)
产品货号	ABT2044
免疫原	合成多肽
宿主	小鼠
反应性	哺乳动物#细菌
标签	HA
检测类型	IP
克隆类型	单克隆
亚型	小鼠IgG1
纯化工艺	通过使用特异性免疫原的亲和层析，从小鼠腹水中纯化抗体。
偶联物	磁珠
产品形式	液体形式
储存缓冲液	PBS缓冲液（pH 7.4），含有0.02％叠氮化钠（防腐剂）。
保存建议	从发货之日起，4°C可稳定保存一年。避免反复冻融或者离心。
运输条件	冰袋运输（蓝冰）
警告	本文列出的产品仅供研究使用，不适用于人类或临床诊断。我们产品所推荐应用，不是建议使用我们的产品去违反任何专利或许可证。对于使用本产品可能发生的专利侵权或其他违规行为，我们不承担任何责任。

使用说明

Reagent Required but Not Supplied

Elution Buffer: 0.1 M Glycine-HCl pH 3.0.

Elution Buffer:

Neutralization Buffer: 1 M Tris-HCl, pH 8.5.

Neutralization Buffer:

Assay Procedure

A. Preparation of magnetic beads

Note: Per 500 μL of protein sample add 20 μL Magnetic Beads. Perform the following procedures, according to add 20 μL Magnetic Beads.

Note:

Add Magnetic Beads to a 1.5 mL centrifuge tube. Place the centrifuge tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant.
Add 1 mL 1×TBS to re-suspend Magnetic Beads, place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant, repeat 3 times. Add 20 μL 1×TBS to re-suspend Magnetic Beads.

Add Magnetic Beads to a 1.5 mL centrifuge tube. Place the centrifuge tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant.

Add 1 mL 1×TBS to re-suspend Magnetic Beads, place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant, repeat 3 times. Add 20 μL 1×TBS to re-suspend Magnetic Beads.

B. Immunoprecipitation

Add 500 μL protein samples to the processed Magnetic Beads, and incubate at room temperature for 1-2 h or overnight at 4℃ (It is recommended to use vertical rotating mixer with Low-speed rotation).
Place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant.
Add 1 mL 1×TBS, and re-suspend Magnetic Beads, place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant, repeat 3-5 times, until OD280 of the supernatant is lesser than 0.05.
Elution
1. Denatured elution: This method is suitable for SDS-PAGE and Western Blotting analysis of elution samples. Add 100 μL (5 times volume of Beads) 1×SDS-PAGE Loading Buffer to the tube and mix well, incubate at 100℃ for 5 min, then Centrifuge at 800 rpm for 1 min, and collect the supernatant to a new tube for SDS-PAGE and Western Blotting analysis.
2. Competitive elution of peptide: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) HA Peptide (0.1-0.2 μg/mL) to the tube and mix well, incubate at 4℃ for 1-2 h (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube. In order to improve the elution efficiency, the incubation time can be Increased or repeat elution. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.
3. Acid elution: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) Elution Buffer to the tube and mix well, incubate at room temperature for 5-10 min (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube, and immediately add 10 μL Neutralization Buffer to adjust the pH to 7.0-8.0. In order to improve the elution efficiency, elution can be repeated, and combine the same samples. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.

Add 500 μL protein samples to the processed Magnetic Beads, and incubate at room temperature for 1-2 h or overnight at 4℃ (It is recommended to use vertical rotating mixer with Low-speed rotation).

Place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant.

Add 1 mL 1×TBS, and re-suspend Magnetic Beads, place the tube on a Magnetic Separation Rack, let stand for 10 s, remove the supernatant, repeat 3-5 times, until OD280 of the supernatant is lesser than 0.05.

Elution

Denatured elution: This method is suitable for SDS-PAGE and Western Blotting analysis of elution samples. Add 100 μL (5 times volume of Beads) 1×SDS-PAGE Loading Buffer to the tube and mix well, incubate at 100℃ for 5 min, then Centrifuge at 800 rpm for 1 min, and collect the supernatant to a new tube for SDS-PAGE and Western Blotting analysis.
Competitive elution of peptide: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) HA Peptide (0.1-0.2 μg/mL) to the tube and mix well, incubate at 4℃ for 1-2 h (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube. In order to improve the elution efficiency, the incubation time can be Increased or repeat elution. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.
Acid elution: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) Elution Buffer to the tube and mix well, incubate at room temperature for 5-10 min (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube, and immediately add 10 μL Neutralization Buffer to adjust the pH to 7.0-8.0. In order to improve the elution efficiency, elution can be repeated, and combine the same samples. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.

Elution

Denatured elution: This method is suitable for SDS-PAGE and Western Blotting analysis of elution samples. Add 100 μL (5 times volume of Beads) 1×SDS-PAGE Loading Buffer to the tube and mix well, incubate at 100℃ for 5 min, then Centrifuge at 800 rpm for 1 min, and collect the supernatant to a new tube for SDS-PAGE and Western Blotting analysis.
Competitive elution of peptide: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) HA Peptide (0.1-0.2 μg/mL) to the tube and mix well, incubate at 4℃ for 1-2 h (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube. In order to improve the elution efficiency, the incubation time can be Increased or repeat elution. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.
Acid elution: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) Elution Buffer to the tube and mix well, incubate at room temperature for 5-10 min (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube, and immediately add 10 μL Neutralization Buffer to adjust the pH to 7.0-8.0. In order to improve the elution efficiency, elution can be repeated, and combine the same samples. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.

Denatured elution: This method is suitable for SDS-PAGE and Western Blotting analysis of elution samples. Add 100 μL (5 times volume of Beads) 1×SDS-PAGE Loading Buffer to the tube and mix well, incubate at 100℃ for 5 min, then Centrifuge at 800 rpm for 1 min, and collect the supernatant to a new tube for SDS-PAGE and Western Blotting analysis.

Denatured elution:

Competitive elution of peptide: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) HA Peptide (0.1-0.2 μg/mL) to the tube and mix well, incubate at 4℃ for 1-2 h (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube. In order to improve the elution efficiency, the incubation time can be Increased or repeat elution. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.

Competitive elution of peptide:

Acid elution: This method can maintain their original biological activity, elution can be used for functional analysis. Add 100 μL (5 times volume of Beads) Elution Buffer to the tube and mix well, incubate at room temperature for 5-10 min (It is recommended to use vertical rotating mixer with Low-speed rotation), then centrifuge at 800 rpm for 2 min at 4℃, and collect the supernatant which is HA-Tag protein and its complex to a new tube, and immediately add 10 μL Neutralization Buffer to adjust the pH to 7.0-8.0. In order to improve the elution efficiency, elution can be repeated, and combine the same samples. Place HA-Tag protein and its complex on ice to be used, or store at -20℃ /-80℃ for long-term. It is recommended to add 100 μL 1×SDS-PAGE Loading Buffer to beads precipitation to test the effect of immunoprecipitation and elution.

Acid elution:

Note: a) For a few samples, due to differences in target proteins, the binding of HA-Tag and Anti-HA antibody is very strong, and the effect of Acid elution and Competitive elution of peptide may be poor. Therefore, SDS-PAGE Loading Buffer denaturation elution method is recommended as a priority; b) Due to the difference of target protein, the elution efficiency of acid elution method also varies to some extent. If the requirement of elution efficiency is high, the pH value of acidic eluent can be adjusted appropriately between 2.5-3.1, and the pH value or quantity of corresponding neutralizing solution should be adjusted appropriately. For example, 100 μL Acid Elution Buffer (0.1 M Glycine-HCl, pH 2.8) and 15 μL Neutralizing Buffer (1 M Tris-HCl, pH 8.5).

Note:

Recommended Products

Catalog No.	Product Name
ABT2014	Magnetic Beads Conjugated Anti-DDDDK Tag Mouse Monoclonal Antibody (1B10)
ABT2024	Magnetic Beads Conjugated Anti-GFP Tag Mouse Monoclonal Antibody (3D3)
ABT2054	Magnetic Beads Conjugated Anti-His Tag Mouse Monoclonal Antibody (5C3)
ABT2064	Magnetic Beads Conjugated Anti-Myc Tag Mouse Monoclonal Antibody (2D5)
ABT2174	Magnetic Beads Conjugated Anti-V5 Tag Mouse Monoclonal Antibody (11D5)

Catalog No.Product NameCatalog No.Product NameABT2014Magnetic Beads Conjugated Anti-DDDDK Tag Mouse Monoclonal Antibody (1B10)ABT2014Magnetic Beads Conjugated Anti-DDDDK Tag Mouse Monoclonal Antibody (1B10)ABT2024Magnetic Beads Conjugated Anti-GFP Tag Mouse Monoclonal Antibody (3D3)ABT2024Magnetic Beads Conjugated Anti-GFP Tag Mouse Monoclonal Antibody (3D3)ABT2054Magnetic Beads Conjugated Anti-His Tag Mouse Monoclonal Antibody (5C3)ABT2054Magnetic Beads Conjugated Anti-His Tag Mouse Monoclonal Antibody (5C3)ABT2064Magnetic Beads Conjugated Anti-Myc Tag Mouse Monoclonal Antibody (2D5)ABT2064Magnetic Beads Conjugated Anti-Myc Tag Mouse Monoclonal Antibody (2D5)ABT2174Magnetic Beads Conjugated Anti-V5 Tag Mouse Monoclonal Antibody (11D5)ABT2174Magnetic Beads Conjugated Anti-V5 Tag Mouse Monoclonal Antibody (11D5)

Disclaimer

The reagent is only used in the field of scientific research, not suitable for clinical diagnosis or other purposes.

常见问题

Q: 普通荧光二抗能不能做WB呢？应该如何成像呢？

A: 荧光western blotting的结果需要特殊的仪器检测，即一种荧光成像仪器。即运用荧光成像仪可以对荧光WB的实验结果进行成像和数据采集分析。如果希望应用荧光成像做WB，建议选用Abbkine DyLight 680和DyLight 800荧光二抗，货号分别为A23710、A23720、A23910、A23920。

Q: Abbkine品牌的二抗的浓度为多少呢？

A: 0.5 mg/ml。

Q: 抗体中甘油的作用是什么？

A: 甘油是可以减慢抗体分子之间的碰撞，起到抗体保护剂的作用。

文献引用

Exercise‐Mediated Mechanical Stress Promotes Osteogenic Differentiation of BMSCs Through Upregulation of Lactylation via the IER3/LDHB Axis.

杂志名称: The FASEB Journal | 作者: Dai, Shuo, et al.

IF: | 发表时间: 2025

专业技术支持

我们的技术团队为您提供全方位的产品支持服务

实验方案设计

根据您的研究目标，提供个性化的实验设计方案

问题排查

经验丰富的技术专家协助您解决实验中遇到的问题

在线技术咨询

7x24小时在线技术支持，随时为您答疑解惑

免费样品申请

提供免费样品试用，让您先试后买更放心

分享产品