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- 详细信息
- 技术资料
- 样本:
液体
- 标记物:
HSP-70
- 适应物种:
不限
- 应用:
科研单位
- 检测方法:
酶联免疫法
- 检测范围:
不限
- 供应商:
瓦兰生物
- 库存:
大量
- 规格:
96T
兔热休克蛋白70(HSP-70)ELISA试剂盒
试剂盒组成
注:标准品浓度依次为:20、10、5、2.5、1.25、0 ng/mL.
试剂的准备
20×洗涤缓冲液的稀释:蒸馏水按1:20稀释,即1份的20×洗涤缓冲液加19份的蒸馏水。
洗板方法
绘制标准曲线:在Excel工作表中,以标准品浓度作横坐标,对应OD值作纵坐标,绘制出标准品线性回归曲线,按曲线方程计算各样本浓度值。
试剂盒性能
上海瓦兰生物科技有限公司售出产品提供售后服务,保证产品质量。凡够买我公司ELISA检测试剂盒可免费提供代测服务。
(以信誉求发展,以质量求生存)
ELISA酶联免疫试剂盒特异性好,灵敏度高。
它的方法类型和操作步骤如下:ELISA可用于测定抗原,也可用于测定抗体。在这种测定方法中有3种必要的试剂:①固相的抗原或抗体,②酶标记的抗原或抗体,③酶作用的底物。根据试剂的来源和标本的性状以及检测的具备条件,可设计出各种不同类型的检测方法。
(一)双抗体夹心法
双抗体夹心法:是检测抗原最常用的方法,操作步骤如下:
(1)将特异性抗体与固相载体连接,形成固相抗体:洗涤除去未结合的抗体及杂质。
(2)加受检标本:使之与固相抗体接触反应一段时间,让标本中的抗原与固相载体上的抗体结合,形成固相抗原复合物。洗涤除去其他未结合的物质。
(3)加酶标抗体:使固相免疫复合物上的抗原与酶标抗体结合。彻底洗涤未结合的酶标抗体。此时固相载体上带有的酶量与标本中受检物质的量正相关。
(4)加底物:夹心式复合物中的酶催化底物成为有色产物。根据颜色反应的程度进行该抗原的定性或定量。
根据同样原理,将大分子抗原分别制备固相抗原和酶标抗原结合物,即可用双抗原夹心法测定标本中的抗体。
(二)双位点一步法
在双抗体夹心法测定抗原时,如应用针对抗原分子上两个不同抗原决定簇的单克隆抗体分别作为固相抗体和酶标抗体,则在测定时可使标本的加入和酶标抗体的加入两步并作一步。这种双位点一步不但简化了操作,缩短了反应时间,如应用高亲和力的单克隆抗体,测定的敏感性和特异性也显著提高。单克隆抗体的应用使测定抗原的ELISA提高到新水平。
在一步法测定中,应注意钩状效应(hookeffect),类同于沉淀反应中抗原过剩的后带现象。当标本中待测抗原浓度相当高时,过量抗原分别和固相抗体及酶标抗体结合,而不再形成夹心复合物,所得结果将低于实际含量。钩状效应严重时甚至可出现假阴性结果。
(三)间接法测抗体
间接法是检测抗体最常用的方法,其原理为利用酶标记的抗抗体以检测已与固相结合的受检抗体,故称为间接法。操作步骤如下:
(1)将特异性抗原与固相载体连接,形成固相抗原:洗涤除去未结合的抗原及杂质。
(2)加稀释的受检血清:其中的特异抗体与抗原结合,形成固相抗原抗体复合物。经洗涤后,固相载体上只留下特异性抗体。其他免疫球蛋白及血清中的杂质由于不能与固相抗原结合,在洗涤过程中被洗去。
(3)加酶标抗抗体:与固相复合物中的抗体结合,从而使该抗体间接地标记上酶。洗涤后,固相载体上的酶量就代表特异性抗体的量。例如欲测人对某种疾病的抗体,可用酶标羊抗人IgG抗体。
每个试剂盒操作是不同的,请按说明书操作。具体事项请来电咨询!
appear uniform, gently tap the plate to ensure thorough mixing.
8. Read the Optical Density (O.D.) at 450 nm using a microtiter plate reader within 15 minutes.
Calculation of results
Storage: 2-8℃.
validity: six months.
FOR RESEARCH USE ONLY; NOT FOR THERAPEUTIC OR DIAGNOSTIC APPLICATIONS! PLEASE READ THROUGH ENTIRE PROCEDURE BEFORE BEGINNING!
试剂盒组成
| 名称 | 96孔配置 | 48孔配置 | 备注 |
| 微孔酶标板 | 12孔×8条 | 12孔×4条 | 无 |
| 标准品 | 0.3mL | 0.3mL | 无 |
| 样本稀释液 | 6mL | 3mL | 无 |
| 检测抗体-HRP | 10mL | 5mL | 无 |
| 20×洗涤缓冲液 | 25mL | 15mL | 按说明书进行稀释 |
| 底物A | 6mL | 3mL | 无 |
| 底物B | 6mL | 3mL | 无 |
| 终止液 | 6mL | 3mL | 无 |
| 封板膜 | 2张 | 2张 | 无 |
| 说明书 | 1份 | 1份 | 无 |
| 自封袋 | 1个 | 1个 | 无 |
试剂的准备
20×洗涤缓冲液的稀释:蒸馏水按1:20稀释,即1份的20×洗涤缓冲液加19份的蒸馏水。
洗板方法
- 手工洗板:甩尽孔内液体,每孔加满洗涤液,静置1min后甩尽孔内液体,在吸水纸上拍干,如此洗板5次。
- 自动洗板机:每孔注入洗液350μL,浸泡1min,洗板5次。
- 从室温平衡60min后的铝箔袋中取出所需板条,剩余板条用自封袋密封放回4℃。
- 设置标准品孔和样本孔,标准品孔各加不同浓度的标准品50μL;
- 待测样本孔先加待测样本10μL,再加样本稀释液40μL;
- 随后标准品孔和样本孔中每孔加入辣根过氧化物酶(HRP)标记的检测抗体100μL,用封板膜封住反应孔,37℃水浴锅或恒温箱温育60min。
- 弃去液体,吸水纸上拍干,每孔加满洗涤液,静置1min,甩去洗涤液,吸水纸上拍干,如此重复洗板5次(也可用洗板机洗板)。
- 每孔加入底物A、B各50μL,37℃避光孵育15min。
- 每孔加入终止液50μL,15min内,在450nm波长处测定各孔的OD值。
绘制标准曲线:在Excel工作表中,以标准品浓度作横坐标,对应OD值作纵坐标,绘制出标准品线性回归曲线,按曲线方程计算各样本浓度值。
试剂盒性能
- 准确性:标准品线性回归与预期浓度相关系数R值,大于等于0.9900。
- 灵敏度:最低检测浓度小于0.1 ng/mL。
- 特异性:不与其它可溶性结构类似物交叉反应。
- 重复性:板内变异系数小于10%、板间变异系数小于15%。
- 贮藏:2-8℃,避光防潮保存。
- 有效期:6个月
- 试剂盒仅供研究使用,不得用于临床实验或人体实验,否则所产生的一切后果,由实验者承担,本公司概不负责。
- 严格按照说明书操作,实验者违反说明书操作,后果由实验者承担。
上海瓦兰生物科技有限公司售出产品提供售后服务,保证产品质量。凡够买我公司ELISA检测试剂盒可免费提供代测服务。
(以信誉求发展,以质量求生存)
ELISA酶联免疫试剂盒特异性好,灵敏度高。
它的方法类型和操作步骤如下:ELISA可用于测定抗原,也可用于测定抗体。在这种测定方法中有3种必要的试剂:①固相的抗原或抗体,②酶标记的抗原或抗体,③酶作用的底物。根据试剂的来源和标本的性状以及检测的具备条件,可设计出各种不同类型的检测方法。
(一)双抗体夹心法
双抗体夹心法:是检测抗原最常用的方法,操作步骤如下:
(1)将特异性抗体与固相载体连接,形成固相抗体:洗涤除去未结合的抗体及杂质。
(2)加受检标本:使之与固相抗体接触反应一段时间,让标本中的抗原与固相载体上的抗体结合,形成固相抗原复合物。洗涤除去其他未结合的物质。
(3)加酶标抗体:使固相免疫复合物上的抗原与酶标抗体结合。彻底洗涤未结合的酶标抗体。此时固相载体上带有的酶量与标本中受检物质的量正相关。
(4)加底物:夹心式复合物中的酶催化底物成为有色产物。根据颜色反应的程度进行该抗原的定性或定量。
根据同样原理,将大分子抗原分别制备固相抗原和酶标抗原结合物,即可用双抗原夹心法测定标本中的抗体。
(二)双位点一步法
在双抗体夹心法测定抗原时,如应用针对抗原分子上两个不同抗原决定簇的单克隆抗体分别作为固相抗体和酶标抗体,则在测定时可使标本的加入和酶标抗体的加入两步并作一步。这种双位点一步不但简化了操作,缩短了反应时间,如应用高亲和力的单克隆抗体,测定的敏感性和特异性也显著提高。单克隆抗体的应用使测定抗原的ELISA提高到新水平。
在一步法测定中,应注意钩状效应(hookeffect),类同于沉淀反应中抗原过剩的后带现象。当标本中待测抗原浓度相当高时,过量抗原分别和固相抗体及酶标抗体结合,而不再形成夹心复合物,所得结果将低于实际含量。钩状效应严重时甚至可出现假阴性结果。
(三)间接法测抗体
间接法是检测抗体最常用的方法,其原理为利用酶标记的抗抗体以检测已与固相结合的受检抗体,故称为间接法。操作步骤如下:
(1)将特异性抗原与固相载体连接,形成固相抗原:洗涤除去未结合的抗原及杂质。
(2)加稀释的受检血清:其中的特异抗体与抗原结合,形成固相抗原抗体复合物。经洗涤后,固相载体上只留下特异性抗体。其他免疫球蛋白及血清中的杂质由于不能与固相抗原结合,在洗涤过程中被洗去。
(3)加酶标抗抗体:与固相复合物中的抗体结合,从而使该抗体间接地标记上酶。洗涤后,固相载体上的酶量就代表特异性抗体的量。例如欲测人对某种疾病的抗体,可用酶标羊抗人IgG抗体。
每个试剂盒操作是不同的,请按说明书操作。具体事项请来电咨询!
Sample collection and storages
Serum - Use a serum separator tube and allow samples to clot for 30 minutes before centrifugation for 10 minutes at approximately 3000×g. Remove serum and assay immediately or aliquot and store samples at -20℃ or -80℃.Avoid repeated freeze-thaw cycles
Plasma - Collect plasma using EDTA or heparin as an anticoagulant. Centrifuge samples for 30 minutes at 3000×g at 2-8℃ within 30 minutes of collection. Store samples at -20℃or -80℃. Avoid repeated freeze-thaw cycles.
Cell culture supernates and other biological fluids - Remove particulates by centrifugation and assay immediately or aliquot and store samples at -20℃or -80℃. Avoid repeated freeze-thaw cycles.
Note: The samples should be centrifugated adequately and no hemolysis or granule was allowed.
Materials required but not supplied
1. Standard microplate reader(450nm)
2. Precision pipettes and Disposable pipette tips.
3. 37 ℃ incubator
Precautions
1. Do not substitute reagents from one kit to another. Standard, conjugate and microplates are matched for optimal performance. Use only the reagents supplied by manufacturer.
2. Do not remove microplate from the storage bag until needed. Unused strips should be stored at 2-8°C in their pouch with the desiccant provided.
3. Mix all reagents before using.
Remove all kit reagents from refrigerator and allow them to reach room temperature ( 20-25°C)
Materials supplied
Note: Standard concentration was followed by:
2400、1200、600、300、150、0 pg/mL.
Reagent preparation
20×wash solution:Dilute with Distilled or deionized water 1:20.
Assay procedure
1. Prepare all reagents before starting assay procedure. It is recommended that all Standards and Samples be added in duplicate to the Microelisa Stripplate.
2. Add standard: Set Standard wells, testing sample wells. Add standard 50μl to standard well.
3. Add Sample: Add testing sample 10μl Then add sample diluent 40μl to testing sample well; Blank well doesn’t add anyting.
4. Add 100μl of HRP-conjugate reagent to each well, cover with an adhesive strip and incubate for 60 minutes at 37°C.
5. Aspirate each well and wash, repeating the process four times for a total of five washes. Wash by filling each well with Wash Solution (400μl) using a squirt bottle, manifold dispenser or autowasher. Complete removal of liquid at each step is essential to good performance. After the last wash, remove any remaining Wash Solution by aspirating or decanting. Invert the plate and blot it against clean paper towels.
6. Add chromogen solution A 50μl and chromogen solution B 50μl to each well. Gently mix and incubate for 15 minutes at 37°C. Protect from light.
7. Add 50μl Stop Solution to each well. The color in the wells should change from blue to yellow. If the color in the wells is green or the color change does not
Serum - Use a serum separator tube and allow samples to clot for 30 minutes before centrifugation for 10 minutes at approximately 3000×g. Remove serum and assay immediately or aliquot and store samples at -20℃ or -80℃.Avoid repeated freeze-thaw cycles
Plasma - Collect plasma using EDTA or heparin as an anticoagulant. Centrifuge samples for 30 minutes at 3000×g at 2-8℃ within 30 minutes of collection. Store samples at -20℃or -80℃. Avoid repeated freeze-thaw cycles.
Cell culture supernates and other biological fluids - Remove particulates by centrifugation and assay immediately or aliquot and store samples at -20℃or -80℃. Avoid repeated freeze-thaw cycles.
Note: The samples should be centrifugated adequately and no hemolysis or granule was allowed.
Materials required but not supplied
1. Standard microplate reader(450nm)
2. Precision pipettes and Disposable pipette tips.
3. 37 ℃ incubator
Precautions
1. Do not substitute reagents from one kit to another. Standard, conjugate and microplates are matched for optimal performance. Use only the reagents supplied by manufacturer.
2. Do not remove microplate from the storage bag until needed. Unused strips should be stored at 2-8°C in their pouch with the desiccant provided.
3. Mix all reagents before using.
Remove all kit reagents from refrigerator and allow them to reach room temperature ( 20-25°C)
Materials supplied
| Name | 96 determinations | 48 determinations |
| Microelisa stripplate | 12*8strips | 12*4strips |
| Standard | 0.3ml | 0.3ml |
| Sample diluent | 6.0ml | 3.0ml |
| HRP-Conjugate reagent | 10.0ml | 5.0ml |
| 20X Wash solution | 25ml | 15ml |
| Chromogen Solution A | 6.0ml | 3.0ml |
| Chromogen Solution B | 6.0ml | 3.0ml |
| Stop Solution | 6.0ml | 3.0ml |
| Closure plate membrane | 2 | 2 |
| User manual | 1 | 1 |
| Sealed bags | 1 | 1 |
2400、1200、600、300、150、0 pg/mL.
Reagent preparation
20×wash solution:Dilute with Distilled or deionized water 1:20.
Assay procedure
1. Prepare all reagents before starting assay procedure. It is recommended that all Standards and Samples be added in duplicate to the Microelisa Stripplate.
2. Add standard: Set Standard wells, testing sample wells. Add standard 50μl to standard well.
3. Add Sample: Add testing sample 10μl Then add sample diluent 40μl to testing sample well; Blank well doesn’t add anyting.
4. Add 100μl of HRP-conjugate reagent to each well, cover with an adhesive strip and incubate for 60 minutes at 37°C.
5. Aspirate each well and wash, repeating the process four times for a total of five washes. Wash by filling each well with Wash Solution (400μl) using a squirt bottle, manifold dispenser or autowasher. Complete removal of liquid at each step is essential to good performance. After the last wash, remove any remaining Wash Solution by aspirating or decanting. Invert the plate and blot it against clean paper towels.
6. Add chromogen solution A 50μl and chromogen solution B 50μl to each well. Gently mix and incubate for 15 minutes at 37°C. Protect from light.
7. Add 50μl Stop Solution to each well. The color in the wells should change from blue to yellow. If the color in the wells is green or the color change does not
appear uniform, gently tap the plate to ensure thorough mixing.
8. Read the Optical Density (O.D.) at 450 nm using a microtiter plate reader within 15 minutes.
Calculation of results
- This standard curve is used to determine the amount in an unknown sample. The standard curve is generated by plotting the average O.D. (450 nm) obtained for each of the six standard concentrations on the vertical (Y) axis versus the corresponding concentration on the horizontal (X) axis.
- First, calculate the mean O.D. value for each standard and sample. All O.D. values, are subtracted by the mean value of the zero standard before result interpretation. Construct the standard curve using graph paper or statistical software.
- To determine the amount in each sample, first locate the O.D. value on the Y-axis and extend a horizontal line to the standard curve. At the point of intersection, draw a vertical line to the X-axis and read the corresponding concentration.
- Any variation in operator, pipetting and washing technique, incubation time or temperature, and kit age can cause variation in result. Each user should obtain their own standard curve.
- The sensitivity by this assay is 10 pg/mL.
- Standard curve
Storage: 2-8℃.
validity: six months.
FOR RESEARCH USE ONLY; NOT FOR THERAPEUTIC OR DIAGNOSTIC APPLICATIONS! PLEASE READ THROUGH ENTIRE PROCEDURE BEFORE BEGINNING!
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兔热休克蛋白70 ( HSP-70 ) ELISA试剂盒
¥2800
