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- 详细信息
- 文献和实验
- 技术资料
- 英文名:
ReadiLink™ Rapid iFluor™ 680 抗体标记试剂盒
- 保存条件:
低温
- 规格:
2 Labelings
ReadiLink™ Rapid iFluor™ 680 抗体标记试剂盒
Components
| Component A: iFluor™ 680 | 2 vials (One vial is for 50 μg protein) |
| Component B: Reaction Buffer | 1 vial (20 μL) |
| Component C: TQ™-Dyed Quench Buffer | 1 vial (20 μL) |
Example protocol
At a glance
Table 1. Available fluorophores in AAT Bioquest ReadyLink™ Rapid Antibody Labelling Kits
| Cat# | Labels | Ex (nm) | Em (nm) |
| 1100 | mFluor™ Violet 450 | 403 | 454 |
| 1105 | mFluor™ Violet 420 | 398 | 411 |
| 1110 | mFluor™ Violet 510 | 414 | 508 |
| 1114 | mFluor™ Violet 540 | 399 | 550 |
| 1120 | mFluor™ Blue 570 | 553 | 570 |
| 1123 | mFluor™ Green 620 | 522 | 617 |
| 1126 | mFluor™ Yellow 630 | 561 | 630 |
| 1130 | mFluor™ Red 700 | 657 | 700 |
| 1131 | mFluor™ Red 780 | 629 | 780 |
| 1220 | iFluor™ 350 | 345 | 442 |
| 1227 | iFluor™ 555 | 559 | 569 |
| 1230 | iFluor™ 594 | 592 | 614 |
| 1235 | iFluor™ 647 | 654 | 674 |
| 1240 | iFluor™ 680 | 682 | 701 |
| 1245 | iFluor™ 700 | 693 | 713 |
| 1250 | iFluor™ 750 | 753 | 779 |
| 1255 | iFluor™ 488 | 491 | 514 |
| 1260 | iFluor™ 633 | 638 | 655 |
| 1265 | iFluor™ 790 | 782 | 811 |
| 1290 | Cy3 | 555 | 565 |
| 1292 | Cy5 | 644 | 665 |
| 1294 | Cy7 | 749 | 776 |
| 1299 | FITC | 494 | 520 |
Preparation of working solution
Important
Warm all the components and centrifuge the vials briefly before opening, and immediately prepare the required solutions before starting your conjugation. The following protocol is for recommendation.
Protein working solution (Solution A):
For labeling 50 µg of protein (assuming the target protein concentration is 1 mg/mL), mix 5 µL (10% of the total reaction volume) of Reaction Buffer (Component B) with 50 µL of the target protein solution. Note: If you have a different protein concentration, adjust the protein volume accordingly to make ~50 µg of protein available for your labeling reaction. Note: For labeling 100 µg of protein (assuming the target protein concentration is 1 mg/mL), mix 10 µL (10% of the total reaction volume) of Reaction Buffer (Component B) with 100 µL of the target protein solution. Note: The protein should be dissolved in 1X phosphate buffered saline (PBS), pH 7.2 - 7.4; if the protein is dissolved in glycine buffer, it must be dialyzed against 1X PBS, pH 7.2 - 7.4, or use Amicon Ultra-0.5, Ultracel-10 Membrane, 10 kDa (cat# UFC501008 from Millipore) to remove free amines or ammonium salts (such as ammonium sulfate and ammonium acetate) that are widely used for protein precipitation. Note: Impure antibodies or antibodies stabilized with bovine serum albumin (BSA) or gelatin will not be labeled well. Note: For optimal labeling efficiency, a final protein concentration range of 1 - 2 mg/mL is recommended, with a significantly reduced conjugation efficiency at less than 1 mg/mL.
Procedure
Run conjugation reaction
- Add the protein working solution (Solution A) to ONE vial of labeling dye (Component A), and mix them well by repeatedly pipetting for a few times or vortex the vial for a few seconds. Note: If labeling 100 µg of protein, use both vials (Component A) of labeling dye by dividing the 100 µg of protein into 2 x 50 µg of protein and reacting each 50 µg of protein with one vial of labeling dye. Then combine both vials for the next step.
- Keep the conjugation reaction mixture at room temperature for 30 - 60 minutes. Note: The conjugation reaction mixture can be rotated or shaken for longer time if desired.
Stop Conjugation reaction
- Add 5 µL (for 50 µg protein) or 10 µL (for 100 µg protein) which is 10% of the total reaction volume of TQ™-Dyed Quench Buffer (Component C) into the conjugation reaction mixture; mix well.
- Incubate at room temperature for 10 minutes. The labeled protein (antibody) is now ready to use.
Storage of Protein Conjugate
The protein conjugate should be stored at > 0.5 mg/mL in the presence of a carrier protein (e.g., 0.1% bovine serum albumin). For longer storage, the protein conjugates could be lyophilized or divided into single-used aliquots and stored at ≤ –20°C.
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文献和实验生物技术有限公司自2007年开始以结核抗体基因检测技术进行结核试剂盒开发研究,并以金标免疫层析阵列技术检测结核病人的血清抗体,从技术层面解决了结核分枝杆菌抗体检测特异性不高的问题,而且还利用两种抗原检测的互补效果提高了检测灵敏度。目前,成功研制的结核抗体快速检测(只需5-6分钟)试剂盒获得新器械产品注册证后已进入市场销售,为结核抗体检测提供了一项新的快速检测手段。
SE 活性部分远低于50%(AlexaFluor488微量标记试剂盒产品信息,Invitrogen)。相反,所有Biotium 的CF染料具有相对稳定的胺活性的SE基团型,这比大部分AlexaFluor 染料的SE更耐水解。总体来说,CF染料SE产品一贯的给出更高的标记效率,提供给用户更好的使用价值。选择方案:蓝色(350-450nm处激发) CF 350、Alexa Fluor 350、AMCA等----亮蓝和紫外光激发CF350是类似于Alexa Fluor 350和传统荧光染料AMCA的蓝色
针对同一指标,生化试剂盒和 ELISA 试剂盒的检测结果趋势是一致的吗?
的特异性产生是由于抗原决定簇决定,抗体产生的过程也比较复杂,特别是小分子抗原必须偶联到载体蛋白上才能产生抗体。 ELISA测定结果的表现形式: 物质浓度:单位主要是μg/mL。 二、从微观角度来看 某一物质的抗原决定簇的活性位点(或者抗原抗体特异性结合位点),与化学反应的活性位点可能存在差异。 三、总的来看 针对同一指标,生化试剂盒和ELISA试剂盒的检测结果趋势是正相关、负相关还是不相关的问题,需要更高技术设备和方法,以及大量的实验数据来验证。从原理中也说明了ELISA试剂盒分种属,而生化试剂盒
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