- 询价
- yuanmu
- 科研
- 进口国产
- YM-SQ2136
- 2025年07月11日
企业认证
相关产品推荐更多 >
万千商家帮你免费找货
0 人在求购买到急需产品
- 详细信息
- 文献和实验
- 技术资料
- 库存:
100
- 供应商:
上海远慕生物科技有限公司
- 检测范围:
科研
- 检测方法:
酶联检测
- 应用:
科研实验
- 适应物种:
Human、 Rat、Mouse 、Monkey、Rabbit
- 规格:
48T/96T
关键词:ELISA试剂盒说明书、ELISA检测试剂盒、ELISAkit技术、进口ELISA试剂盒
上海远慕ELISA试剂盒供应商!
Aflatoxin ELISA Kit使用说明书本
规格:48T/96T
货号:YM-SQ2136
全称:黄曲霉毒素(Aflatoxin)ELISA 试剂盒
Aflatoxin ELISA Kit使用说明书本 Kit composition:
Reagent box is composed of 48 holes with 96 well configuration.
Instruction manual 1 1
Plate film 2 (48) 2 (96)
Sealed bag 1 1
The enzyme labeled plate was kept at 1 * 481 * 96 2-8
Standard product: 0.5ml 540ng/ml * 1 0.5ml * 1 2-8
Standard solution 1.5ml * 1 1.5ml * 1 2-8
Enzyme labeled reagent 3 ml * 6 ml * 1 2-8
Sample dilution liquid 3 ml * 6 ml * 1 2-8
Color ml 3 ml 6 A 1 2-8 1
Color ml 3 ml 6 B 1 2-8 1
3l * 1 6ml * 1 2-8
Concentrated washing solution (20ml * 20) * 1 (20ml * 30) x 1 bottles of 2-8
Sample handling and requirements:
1 serum: 10-20 minutes at room temperature and blood natural coagulation, about 20 minutes (2000-3000). Carefully collected supernatant, preserved in the process, such as precipitation, should be re centrifuge.
2. The plasma should be according to the requirements of the specimens of choice of EDTA or sodium citrate as an anticoagulant, 10-20 minutes after mixing, centrifuged for 20 minutes or so (2000-3000 r.p.m.). Carefully collected supernatant, preserved in the process, such as precipitation, it should be re - centrifugal.
3 urine: use sterile tube collection, centrifugal 20 minutes or so (2000-3000). Carefully collected supernatant, preserved in the process, such as precipitation, should be re - centrifugal. Reference to the chest and ascites, cerebrospinal fluid.
4 cell culture supernatant: the collection of sterile tubes for the detection of secretory components. Centrifugal 20 minutes or so (2000-3000 / min).
Carefully collected supernatant. When the cells were detected by PBS (PH7.2-7.4), the cell concentration reached 1000000 /ml. By repeatedly freezing and thawing, so that the cell damage and release of intracellular components. Centrifugal 20 minutes or so (2000-3000 / min). Carefully collected supernatant. In the process of preservation, if there is a precipitate, it should be again.
5 tissue specimens: after cutting the specimen, the weight is weighed. Adding a certain amount of PH7.4, PBS. Quickly frozen with liquid nitrogen. The temperature of the sample was maintained at 2-8. Adding a certain amount of PBS (PH7.4), using the hand or the homogenate of the specimen homogenate.
Centrifugal 20 minutes or so (2000-3000 / min). Carefully collected supernatant. Be detected after a repackaging, remaining frozen spare.
6 samples collected as soon as possible after extraction, extraction by the relevant literature, and then the experiment should be carried out as soon as possible. If the test can not be carried out immediately, the specimen can be kept at -20, but it should be avoided.
7 could not detect the NaN3 containing samples, because NaN3 inhibited the content of horseradish peroxidase (HRP). Operation steps
标准品的稀释与加样:在酶标包被板上设标准品孔10孔,在第一、第二孔中分别加标准品100μl,然后在第一、第二孔中加标准品稀释液50μl,混匀;然后从第一孔、第二孔中各取100μl分别加到第三孔和第四孔,再在第三、第四孔分别加标准品稀释液50μl,混匀;然后在第三孔和第四孔中先各取50μl弃掉,再各取50μl分别加到第五、第六孔中,再在第五、第六孔中分别加标准品稀释液50ul,混匀;混匀后从第五、第六孔中各取50μl分别加到第七、第八孔中,再在第七、第八孔中分别加标准品稀释液50μl,混匀后从第七、第八孔中分别取50μl加到第九、第十孔中,再在第九第十孔分别加标准品稀释液50μl,混匀后从第九第十孔中各取50μl弃掉。 (the L, 240ng/ml,, 60ng/ml,, 30ng/ml,, 360ng/ml,,,, and 120ng/ml, respectively)
Add sample: respectively, the blank hole (blank control hole without the sample and the enzyme label, and the remaining steps are the same), the sample hole. In the enzyme standard coated plate to be tested on a sample hole Zhongxian sample dilution of 40 g l, and then to be measured is added 10 mu l of sample (sample final dilution degrees for 5 times). The sample will be added to the bottom of the plate hole, and the hole wall is not to be touched.
Temperature: 37 minutes after the closure of the sealing plate with a sealing plate.
With liquid: 30 (48T 20 times) times concentrated washing liquid with distilled water 20 (48T 30 times) after dilution.
Washing: be careful torn off the seal plate membrane, discard liquid, drying, washing liquid to fill each hole, standing for 30 seconds after the discard, repeat 5 times, pat dry.
Add enzyme: 50 L per hole, except for the blank.
Wen Yu: operation with 3.
Washing: operation with 5.
Color: each hole first add color agent A50 L, and then add color agent B50 L, gently shake mix well, 37 to 15 minutes.
Termination: termination of 50 L per hole, terminate the reaction (at this time, blue).
Determination: the blank absorbance at 450nm air conditioning zero, in order to measure the hole (OD). Determination should be carried out within 15 minutes after the termination of the liquid.
Note:
Kit from the cold storage environment in the room temperature balance 15-30 minutes after the use of the enzyme labeled package is not used up after the Kaifeng, the plate should be stored in a sealed bag.
Washing buffer will crystallization, heated the water solubilization when diluted, washing does not affect the results.
Each step should be used with the sample, and often to check the accuracy, to avoid the test error. A sample within 5 mins, ifthenumberofsampleismuch, recommend to use volley like.
Please do the standard curve at the same time, it is best to do the hole. Such as samples to be measured matter content is too high (the sample od is bigger than the first standard hole hole OD), please first sample dilution multiples (n times) were measured and calculated please then multiplied by the total dilution ratio (n * * 5).
Closure plate membrane for one-time use, to avoid cross contamination.
Substrate please avoid light preservation.
In strict accordance with the instructions of the operation, the test results must be determined by the reader's reading.
All samples, washing liquid and all kinds of waste should be treated according to the transmission.
This reagent not mix different batches.
10 if there is a different from the instruction of the English language, the English instruction manual shall prevail.
Calculation:
To the standard concentration as the abscissa, OD value as the ordinate, draw the standard curve on coordinate paper, according to the OD value of samples from the standard curve found corresponding concentration; multiply again
Kit performance:
1 sample linear regression with the expected concentration correlation coefficient R value is 0.92 above.
The 2 batch and batch shall be less than 9% and 15% respectively.
Detection range:
-480ng/ml 12ng/ml
Preservation conditions and validity:
1 Kit: 2-8.
2 validity: 6 months
黄曲霉毒素(Aflatoxin)ELISA 试剂盒
上海远慕ELISA试剂盒供应商!
Aflatoxin ELISA Kit使用说明书本
规格:48T/96T
货号:YM-SQ2136
全称:黄曲霉毒素(Aflatoxin)ELISA 试剂盒
Aflatoxin ELISA Kit使用说明书本 Kit composition:
Reagent box is composed of 48 holes with 96 well configuration.
Instruction manual 1 1
Plate film 2 (48) 2 (96)
Sealed bag 1 1
The enzyme labeled plate was kept at 1 * 481 * 96 2-8
Standard product: 0.5ml 540ng/ml * 1 0.5ml * 1 2-8
Standard solution 1.5ml * 1 1.5ml * 1 2-8
Enzyme labeled reagent 3 ml * 6 ml * 1 2-8
Sample dilution liquid 3 ml * 6 ml * 1 2-8
Color ml 3 ml 6 A 1 2-8 1
Color ml 3 ml 6 B 1 2-8 1
3l * 1 6ml * 1 2-8
Concentrated washing solution (20ml * 20) * 1 (20ml * 30) x 1 bottles of 2-8
Sample handling and requirements:
1 serum: 10-20 minutes at room temperature and blood natural coagulation, about 20 minutes (2000-3000). Carefully collected supernatant, preserved in the process, such as precipitation, should be re centrifuge.
2. The plasma should be according to the requirements of the specimens of choice of EDTA or sodium citrate as an anticoagulant, 10-20 minutes after mixing, centrifuged for 20 minutes or so (2000-3000 r.p.m.). Carefully collected supernatant, preserved in the process, such as precipitation, it should be re - centrifugal.
3 urine: use sterile tube collection, centrifugal 20 minutes or so (2000-3000). Carefully collected supernatant, preserved in the process, such as precipitation, should be re - centrifugal. Reference to the chest and ascites, cerebrospinal fluid.
4 cell culture supernatant: the collection of sterile tubes for the detection of secretory components. Centrifugal 20 minutes or so (2000-3000 / min).
Carefully collected supernatant. When the cells were detected by PBS (PH7.2-7.4), the cell concentration reached 1000000 /ml. By repeatedly freezing and thawing, so that the cell damage and release of intracellular components. Centrifugal 20 minutes or so (2000-3000 / min). Carefully collected supernatant. In the process of preservation, if there is a precipitate, it should be again.
5 tissue specimens: after cutting the specimen, the weight is weighed. Adding a certain amount of PH7.4, PBS. Quickly frozen with liquid nitrogen. The temperature of the sample was maintained at 2-8. Adding a certain amount of PBS (PH7.4), using the hand or the homogenate of the specimen homogenate.
Centrifugal 20 minutes or so (2000-3000 / min). Carefully collected supernatant. Be detected after a repackaging, remaining frozen spare.
6 samples collected as soon as possible after extraction, extraction by the relevant literature, and then the experiment should be carried out as soon as possible. If the test can not be carried out immediately, the specimen can be kept at -20, but it should be avoided.
7 could not detect the NaN3 containing samples, because NaN3 inhibited the content of horseradish peroxidase (HRP). Operation steps
标准品的稀释与加样:在酶标包被板上设标准品孔10孔,在第一、第二孔中分别加标准品100μl,然后在第一、第二孔中加标准品稀释液50μl,混匀;然后从第一孔、第二孔中各取100μl分别加到第三孔和第四孔,再在第三、第四孔分别加标准品稀释液50μl,混匀;然后在第三孔和第四孔中先各取50μl弃掉,再各取50μl分别加到第五、第六孔中,再在第五、第六孔中分别加标准品稀释液50ul,混匀;混匀后从第五、第六孔中各取50μl分别加到第七、第八孔中,再在第七、第八孔中分别加标准品稀释液50μl,混匀后从第七、第八孔中分别取50μl加到第九、第十孔中,再在第九第十孔分别加标准品稀释液50μl,混匀后从第九第十孔中各取50μl弃掉。 (the L, 240ng/ml,, 60ng/ml,, 30ng/ml,, 360ng/ml,,,, and 120ng/ml, respectively)
Add sample: respectively, the blank hole (blank control hole without the sample and the enzyme label, and the remaining steps are the same), the sample hole. In the enzyme standard coated plate to be tested on a sample hole Zhongxian sample dilution of 40 g l, and then to be measured is added 10 mu l of sample (sample final dilution degrees for 5 times). The sample will be added to the bottom of the plate hole, and the hole wall is not to be touched.
Temperature: 37 minutes after the closure of the sealing plate with a sealing plate.
With liquid: 30 (48T 20 times) times concentrated washing liquid with distilled water 20 (48T 30 times) after dilution.
Washing: be careful torn off the seal plate membrane, discard liquid, drying, washing liquid to fill each hole, standing for 30 seconds after the discard, repeat 5 times, pat dry.
Add enzyme: 50 L per hole, except for the blank.
Wen Yu: operation with 3.
Washing: operation with 5.
Color: each hole first add color agent A50 L, and then add color agent B50 L, gently shake mix well, 37 to 15 minutes.
Termination: termination of 50 L per hole, terminate the reaction (at this time, blue).
Determination: the blank absorbance at 450nm air conditioning zero, in order to measure the hole (OD). Determination should be carried out within 15 minutes after the termination of the liquid.
Note:
Kit from the cold storage environment in the room temperature balance 15-30 minutes after the use of the enzyme labeled package is not used up after the Kaifeng, the plate should be stored in a sealed bag.
Washing buffer will crystallization, heated the water solubilization when diluted, washing does not affect the results.
Each step should be used with the sample, and often to check the accuracy, to avoid the test error. A sample within 5 mins, ifthenumberofsampleismuch, recommend to use volley like.
Please do the standard curve at the same time, it is best to do the hole. Such as samples to be measured matter content is too high (the sample od is bigger than the first standard hole hole OD), please first sample dilution multiples (n times) were measured and calculated please then multiplied by the total dilution ratio (n * * 5).
Closure plate membrane for one-time use, to avoid cross contamination.
Substrate please avoid light preservation.
In strict accordance with the instructions of the operation, the test results must be determined by the reader's reading.
All samples, washing liquid and all kinds of waste should be treated according to the transmission.
This reagent not mix different batches.
10 if there is a different from the instruction of the English language, the English instruction manual shall prevail.
Calculation:
To the standard concentration as the abscissa, OD value as the ordinate, draw the standard curve on coordinate paper, according to the OD value of samples from the standard curve found corresponding concentration; multiply again
Kit performance:
1 sample linear regression with the expected concentration correlation coefficient R value is 0.92 above.
The 2 batch and batch shall be less than 9% and 15% respectively.
Detection range:
-480ng/ml 12ng/ml
Preservation conditions and validity:
1 Kit: 2-8.
2 validity: 6 months
黄曲霉毒素(Aflatoxin)ELISA 试剂盒
风险提示:丁香通仅作为第三方平台,为商家信息发布提供平台空间。用户咨询产品时请注意保护个人信息及财产安全,合理判断,谨慎选购商品,商家和用户对交易行为负责。对于医疗器械类产品,请先查证核实企业经营资质和医疗器械产品注册证情况。
文献和实验相关实验
有替代前者的趋势。由于ABS-ELISA较普通ELISA多用了两种试剂,增加了操作步骤,在临床检验中ABS-ELISA应用不多。科研项目中检测微量的成分如细胞因子常采用本法。晶美分装ELISA KIT采用的方法:1, TORCH及传染病试剂盒(间接法),见2.2.32, TORCH-IgM捕获法特色:包被抗体,标记抗原原理:3, 细胞因子试剂盒采用的方法路线(ABC-ELISA)原理产品特色:采用ABC法,灵敏度更高,特异性更强。生物素抗体和酶联物是浓缩的,使用前需用相应的缓冲液稀释。酶联物可以通用
人脂联素酶联免疫分析ELISA试剂盒使用说明书本试剂盒仅供研究使用产品编号:E0605h 预期应用ELISA法定量测定人血清、血浆、细胞培养物上清或其它相关液体中脂联素含量。实验原理本试剂盒应用双抗体夹心酶标免疫分析法测定标本中脂联素水平。用纯化的抗体包被微孔板,制成固相抗体,往包被单抗的微孔中依次加入脂联素抗原、生物素化的抗人脂联素抗体、HRP标记的亲和素,经过彻底洗涤后用底物TMB显色。TMB在过氧化物酶的催化下转化成蓝色,并在酸的作用下转化成最终的黄色。颜色的深浅和样品中的脂联素呈正相
R&D Systems支原体污染检测新方法(ELISA)专辑
R&D Systems支原体污染检测新方法(ELISA)专辑 不需要特殊仪器,可同时检测8种支原体,并避免支原体检测出现假阴性和假阳性的方法 前言: 支 原体污染是细胞培养中令人头痛的问题,有研究表明25%的细胞系中感染了支原体,而研究人员却并不知晓!支原体检测常规采用PCR的方法,虽然灵敏,但假 阳性和假阴性率高,面对得之不易的细胞,研究人员往往很难取舍。对此,R&D Systems 公司在这个领域有重大突破,利用Elisa技术研发的新产品—MycoProbe®
技术资料暂无技术资料 索取技术资料
Aflatoxin ELISA Kit使用说明书本
询价
