MBTPS2 抗体 MBTPS2 Antibody

MBTPS2 抗体

MBTPS2 Antibody

详细描述:
Species predicted to react based on 100% sequence homology: Human。MBTPS2 Antibody识别内源性的MBTPS2总蛋白。该多克隆抗体用与小鼠MBTPS2序列对应的人工合成肽段免疫动物而制成。该抗体使用蛋白A和蛋白亲和层析纯化而得。MBTPS2 Antibody detects endogenous levels of total MBTPS2 protein.Polyclonal antibodies are produced by immunizing animals with a synthetic peptide corresponding to the sequence of mouse MBTPS2. Antibodies are purified by protein A and peptide affinity chromatography.

应用范围:W; 反应种属:Mouse; 灵敏度:Endogenous; MW (kDa):57; Isotype:Rabbit; 标记:无标记。

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货号 名称 单位 购买
2157S MBTPS2 抗体 100µl 咨询客服

Wakopak Navi C18-5 4.0*250mm 高性能高纯硅胶柱C18-5 品牌:FUJIFILM Wako


Wakopak Navi C18-5 4.0*250mm

高性能高纯硅胶柱C18-5

品牌:FUJIFILM Wako
CAS No.:
储存条件:室温
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

233-60451

1 column(D) 5,920.00


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Wakopak Wakosil-II5C18HG 4.0*250mm 高纯硅胶柱5C18 HG 品牌:FUJIFILM Wako


Wakopak Wakosil-II5C18HG 4.0*250mm

高纯硅胶柱5C18 HG

品牌:FUJIFILM Wako
CAS No.:
储存条件:室温
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

237-51061

1 column(D) 咨询


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DT Cryo-Tags, 1.05in x 0.5in, white打印标签纸 DT Cryo-Tags, 1.05in x 0.5in, white

DT Cryo-Tags, 1.05in x 0.5in, white打印标签纸

DT Cryo-Tags, 1.05in x 0.5in, white

详细描述:
1.05 x 0.50in White 1,000 Labels/Unit Brand: Diversified Biotech

Direct Thermal Cryo-Tags®, 1.05in x 0.50in (27mm x 13mm) Direct Thermal Transfer Labels for 0.5ml Tubes, Roll, White Can withstand temperatures from -196°C to 70°C Also freezable in liquid nitrogen and vapor phase nitrogen Adhere to most plastics, glass and metals without cracking or degrading Set up instructions for PC and Mac users available below! Scroll down to read and also download templates to use with Dymo software!

货号 产品名称 品牌 购买
货号 名称 单位 购买
89-168 DT Cryo-Tags, 1.05in x 0.5in, white打印标签纸 Labels/Unit 咨询客服

VE-Cadherin 抗体 VE-Cadherin Antibody

VE-Cadherin 抗体

VE-Cadherin Antibody

详细描述:
VE-Cadherin抗体可以识别内源性总的VE-cadherin蛋白。抗体与其他cadherin家族成员没有交叉反应。合成对应人VE-cadherin羧基端序列的多肽免疫动物获得多克隆抗体。抗体由蛋白A和肽亲和层析纯化。VE-Cadherin Antibody detects endogenous levels of total VE-cadherin protein. The antibody does not cross-react with other cadherin family members.Polyclonal antibodies are produced by immunizing animals with a synthetic peptide corresponding to the carboxy-terminus of human VE-cadherin. Antibodies are purified by protein A and peptide affinity chromatography.

应用范围:W IF-IC ; 反应种属:Human,D. melanogaster,Bovine; 灵敏度:Endogenous; MW (kDa):130-140; Isotype:Rabbit; 标记:无标记。

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货号 名称 单位 购买
2158S VE-Cadherin 抗体 100µl 咨询客服

Wakopak Wakosil-II5C18RS 4.0*30mm 高纯硅胶柱5C18RS 品牌:FUJIFILM Wako


Wakopak Wakosil-II5C18RS 4.0*30mm

高纯硅胶柱5C18RS

品牌:FUJIFILM Wako
CAS No.:
储存条件:室温
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

236-51391

1 column(D) 咨询


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BstEII-HF(星选酶)–NEB酶试剂

产品资料 – 限制性内切酶 – 高保真限制性内切酶

BstEII-HF(星选酶)                              收藏

BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂 BstEII-HF(星选酶)--NEB酶试剂

货 号
规 格
价 格
北京库存
上海库存
广州库存
成都库存

#R3162L
10,000 units
2,779.00元

#R3162M
(高浓度5X)10,000 units
2,779.00元

#R3162S
2,000 units
659.00元

#R3162V
1,000 units
349.00元

Download:       

识别位点

BstEII-HF(星选酶)--NEB酶试剂

  • isoschizomers     |
  • compatible ends     | 
  • single letter code

在不同反应缓冲液的活性

NEBuffer 1.1: <10%
NEBuffer 2.1: 10%
NEBuffer 3.1: <10%
CutSmart Buffer: 100%

特性

CutSmart、重组酶、基因工程改造酶、省时酶、高保真酶。

反应条件

CutSmart 缓冲液,37℃。

浓度

20,000 和 100,000 units/ml。

甲基化敏感性

dam、dcm 和哺乳动物 CpG 甲基化均不敏感。

注意事项

在已知的 3,000 多种限制性内切酶中,BstEll 是少数几个能够产生多于 4 个碱基突出端的内切酶之一。

DT Cryo-tags, 1.05in x 0.5in, yellow打印标签纸 DT Cryo-tags, 1.05in x 0.5in, yellow

DT Cryo-tags, 1.05in x 0.5in, yellow打印标签纸

DT Cryo-tags, 1.05in x 0.5in, yellow

详细描述:
1.05 x 0.50in White 1,000 Labels/Unit Brand: Diversified Biotech

Direct Thermal Cryo-Tags®, 1.05in x 0.50in (27mm x 13mm) Direct Thermal Transfer Labels for 0.5ml Tubes, Roll, White Can withstand temperatures from -196°C to 70°C Also freezable in liquid nitrogen and vapor phase nitrogen Adhere to most plastics, glass and metals without cracking or degrading Set up instructions for PC and Mac users available below! Scroll down to read and also download templates to use with Dymo software!

货号 产品名称 品牌 购买
货号 名称 单位 购买
89-168Y DT Cryo-tags, 1.05in x 0.5in, yellow打印标签纸 Labels/Unit 咨询客服

Wakopak Wakosil-DNA 4.6*150mm DNA分析柱 品牌:FUJIFILM Wako


Wakopak Wakosil-DNA 4.6*150mm

DNA分析柱

品牌:FUJIFILM Wako
CAS No.:
储存条件:室温
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

239-59321

1 column(D) 咨询


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M13KO7 辅助噬菌体–NEB酶试剂

产品资料 – DNA修饰酶与克隆技术 – 其它

M13KO7 辅助噬菌体                              收藏

货 号
规 格
价 格
北京库存
上海库存
广州库存
成都库存

#N0315S
1.8 ml
1,299.00元

Download:       

  • isoschizomers     |
  • compatible ends     | 
  • single letter code

特性

产生用于测序和突变的单链噬菌粒 DNA 

概述

 
M13KO7 是 M13 噬菌体。其具有 P15A 的复制起点和 Tn903 卡那霉素抗性基因,这两个片段插入 M13 的复制起点。 M13KO7 在没有噬菌粒 DNA的条件下也能复制。当存在一个携带有野生型的M13 或 f1 复制起点的噬菌粒时,单链噬菌粒可以完整包装,并分泌到培养基中。该特性使其便于生产用作突变和测序的单链噬菌粒 DNA。 M13KO7携带卡那霉素抗性标记。

来源

M13KO7 噬菌体上清按照标准程序分离自受侵染的 E. coli ER2738。 

浓度

1.0 X 1011 pfu/ml。 

注意事项

NEB 不推荐将 M13KO7 作为一个克隆载体使用。构建噬菌体展示文库,推荐使用 Ph.D.™ 肽库展示克隆系统(详见 251 页)。 

相关产品

抗 M13 pIII 单克隆抗体

DNMT3A 抗体 DNMT3A Antibody

DNMT3A 抗体

DNMT3A Antibody

详细描述:
Species predicted to react based on 100% sequence homology: Bovine。DNMT3A Antibody能够检测内源性DNMT3A总蛋白水平。该抗体不能与DNMT3B或其它DNMT蛋白发生相互作用。通过合成的与人源DNMT3A蛋白相应的多肽片段去免疫动物从而制备出此多克隆抗体。通过蛋白A和多肽亲和层析纯化获得。DNMT3A Antibody detects endogenous levels of total DNMT3A protein. The antibody does not cross-react with DNMT3B or other DNMT proteins.Polyclonal antibodies are produced by immunizing animals with a synthetic peptide corresponding to the human DNMT3A protein. Antibodies are purified by protein A and peptide affinity chromatography.

应用范围:W IP; 反应种属:Human,Mouse,Rat,Monkey; 灵敏度:Endogenous; MW (kDa):130; Isotype:Rabbit; 标记:无标记。

货号 产品名称 品牌 购买
货号 名称 单位 购买
2160S DNMT3A 抗体 100µl 咨询客服

Oligo d(T)18 mRNA 引物–NEB酶试剂

产品资料 – RNA 试剂 – cDNA 合成

Oligo d(T)18 mRNA 引物                              收藏

货 号
规 格
价 格
北京库存
上海库存
广州库存
成都库存

#S1316S
5.0 A260 units
979.00元

Download:       

  • isoschizomers     |
  • compatible ends     | 
  • single letter code

概述

Oligo d(N)n 引物适用于 mRNA 的扩增和测序,能与 mRNA 的 3´ -poly A 尾或带尾的 cDNA 退火。

注意:#S1316 5´ 末端未磷酸化。

参考文献

有关该产品特性和应用的参考文献请登陆 www.neb-china.com,www.neb.com。

Wakopak Wakosil5C4 4.0*200mm 硅胶柱5C4 品牌:FUJIFILM Wako


Wakopak Wakosil5C4 4.0*200mm

硅胶柱5C4

品牌:FUJIFILM Wako
CAS No.:
储存条件:室温
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

238-56753

1 column(W) 咨询


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膜电位荧光探针DiSBAC2(5) 货号21415-AAT Bioquest荧光染料

上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

膜电位荧光探针DiSBAC2(5)

膜电位荧光探针DiSBAC2(5)

膜电位荧光探针DiSBAC2(5)    货号21415 货号 21415 存储条件 在零下15度以下保存, 避免光照
规格 25 mg 价格 1896
Ex (nm) 636 Em (nm) 655
分子量 462.59 溶剂 DMSO
产品详细介绍

简要概述

膜电位荧光探针DiSBAC2(5)是美国AAT Bioquest生产的用于膜电位检测的荧光探针,DiSBAC2(5)是一种灵敏的慢响应膜电位探针,广泛用于测量许多生物系统的膜电位。通常,慢反应探针显示其跨膜分布的潜在依赖性变化,伴随荧光变化。它们的光学响应的​​幅度远大于快速响应探针的幅度(通常每mV的荧光变化为1%)。包括阳离子羰花青,罗丹明和阴离子氧杂菁的慢反应探针适用于检测由呼吸活动,离子通道渗透性,药物结合和其他因素引起的非激发细胞的平均膜电位的变化。金畔生物是AAT Bioquest的中国代理商,为您提供最优质的膜电位荧光探针DiSBAC2(5)。 

点击查看光谱

产品说明书

操作步骤

1.准备细胞:

1.1对于贴壁细胞:在生长培养基中将细胞以40,000至80,000个细胞/孔/100μL在96孔板中培养过夜,或对于384孔板以10,000至20,000个细胞/孔/25μL。

1.2对于非粘附细胞:从培养基中离心细胞,然后将细胞沉淀悬浮于等量的HHBS和MP染料加载溶液(参见下面的步骤2.2),125,000至250,000细胞/孔/100μL,96-以及聚赖氨酸d板或30,000至60,000个细胞/孔/25μL的用于384孔聚赖氨酸d板。在实验之前,在制动器关闭的情况下以800rpm 离心板2分钟。

注意:每个细胞系应在个人基础上进行评估,以确定最佳的细胞密度为细胞内钙动员。

 

2.准备DiSBAC2(3)染料加载溶液(1板):

2.1在高质量无水DMSO中制备10至30 mM的DiSBAC2(3)原液。应及时使用原液; 任何剩余的溶液需要被等分并冷冻在< -20 ö C.

注意:避免反复冻融循环,避免光照。

2.2制备2X DiSBAC2(3)染料加载 溶液: 在实验当天,将DiSBAC2(3) 固体溶解在DMSO中或将等分试样的DiSBAC2(3)储备溶液解冻至室温。用0.04%的制备的在Hanks(HHBS)20至40μM和20mM Hepes缓冲液或者缓冲您的选择,pH为7的2X工作溶液到0.08%的Pluronic ® F-127(目录#20053)和2mM 锥虫红Plus(Cat#2456)。通过votexing很好地混合它们。该工作溶液在室温下稳定至少2小时。

 

3.运行膜电位测定:

3.1将100μL/孔(96孔板)或25μL/孔(384孔板)DiSBAC2(3)染料加载溶液(来自步骤2.2)加入细胞板中。

注1:如果您的筛选化合物干扰g rowth培养基和血清因子,在添加DiSBAC2(3)染料加载 溶液之前,用等体积的HHBS缓冲液替换生长培养基。或者,细胞可以在无血清条件下生长。

注2:染料加载后不要洗涤细胞。

3.2将染料加载板在细胞培养箱中孵育30至60分钟。

注意:在病例中,在室温下孵育30至60分钟可能会更好。

3.3使用HHBS或所需的缓冲液制备复合板。 

3.4通过监测Ex / Em = 540 / 590nm处的荧光强度(Cat#21414)进行膜电位测定。

注意:在实验之前运行信号测试很重要。不同的仪器有自己的强度范围。将信号测试强度调整到最大仪器强度计数的10%至15%的水平。例如,FLIPR-384的最大荧光强度计数为65,000,因此应调整仪器设置以使其信号测试强度在7,000到10,000左右。 

 

参考文献

Suppression of K V 7/KCNQ potassium channel enhances neuronal differentiation of PC12 cells
Authors: Najing Zhou, Sha Huang, Li Li, Dongyang Huang, Yunli Yan, Xiaona Du, Hailin Zhang
Journal: Neuroscience (2016): 356–367

说明书
膜电位荧光探针DiSBAC2(5).pdf

DT Cryo-Spots, 1/2in diameter, orange打印标签纸 DT Cryo-Spots, 1/2in diameter, orange

DT Cryo-Spots, 1/2in diameter, orange打印标签纸

DT Cryo-Spots, 1/2in diameter, orange

详细描述:
1.05 x 0.50in White 1,000 Labels/Unit Brand: Diversified Biotech

Direct Thermal Cryo-Tags®, 1.05in x 0.50in (27mm x 13mm) Direct Thermal Transfer Labels for 0.5ml Tubes, Roll, White Can withstand temperatures from -196°C to 70°C Also freezable in liquid nitrogen and vapor phase nitrogen Adhere to most plastics, glass and metals without cracking or degrading Set up instructions for PC and Mac users available below! Scroll down to read and also download templates to use with Dymo software!

货号 产品名称 品牌 购买
货号 名称 单位 购买
89-171O DT Cryo-Spots, 1/2in diameter, orange打印标签纸 Labels/Unit 咨询客服

α-N-Catenin (C12G4) 兔单克隆抗体 α-N-Catenin (C12G4) Rabbit mAb

α-N-Catenin (C12G4) 兔单克隆抗体

α-N-Catenin (C12G4) Rabbit mAb

详细描述:
α-N-Catenin (C12G4)兔单抗可以识别内源性总的α-N-catenin蛋白。抗体与其他α-N-catenin家族成员没有交叉反应。合成对应人α-N-Catenin的羧基端序列的多肽免疫动物获得单克隆抗体。α-N-Catenin (C12G4) Rabbit mAb detects endogenous levels of total α-N-catenin protein. The antibody does not cross-react with other α-catenin family members.Monoclonal antibody is produced by immunizing animals with a synthetic peptide corresponding to the carboxy-terminal sequence of human α-N-Catenin.

应用范围:W IP IF-IC; 反应种属:Human,Mouse,Rat; 灵敏度:Endogenous; MW (kDa):102; Isotype:Rabbit IgG; 标记:无标记。

货号 产品名称 品牌 购买
货号 名称 单位 购买
2163S α-N-Catenin (C12G4) 兔单克隆抗体 100µl 咨询客服

Anti 4R-Tau, Monoclonal Antibody(3E8-1A6) 抗4R-Tau,单克隆抗体(3E8-1A6) 品牌:Wako


品牌:Wako
CAS No.:
储存条件:-20℃
纯度:
产品编号

(生产商编号)

等级 规格 运输包装 零售价(RMB) 库存情况 参考值

019-26593

用于免疫组化 10 ul 咨询


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海藻糖检测试剂盒Trehalose Assay Kit Trehalose Assay Kit 货号:K-TREH Megazyme试剂盒

海藻糖检测试剂盒Trehalose Assay Kit

英文名:Trehalose Assay Kit

货号:K-TREH

规格:100 assays (manual) / 1000 assays (microplate)

市场价: 4200

The Trehalose test kit is a simple method for the rapid and reliable measurement and analysis of trehalose in foods, beverages and other materials.

Suitable for manual, auto-analyser and microplate formats.

UV-method for the determination of Trehalose and
D-Glucose in foodstuffs, beverages, and other materials

Principle:
(trehalase)
(1) Trehalose + H2O → D-glucose

(hexokinase)
(2) D-Glucose + ATP → G-6-P + ADP

(glucose-6-phosphate dehydrogenase)
(3) G-6-P + NADP+ → gluconate-6-phosphate + NADPH + H+

Kit size: 100 assays (manual) / 1000 (microplate)
/ 1100 (auto-analyser)
Method: Spectrophotometric at 340 nm
Reaction time: ~ 8 min
Detection limit: 37.5 mg/L
Application examples:
Honey, mushrooms, bread, beer, seafood (e.g. lobster and shrimp),
fruit juices, purees and fillings, nutrition bars, surimi, dehydrated fruits
and vegetables, fruit products, white chocolate, sports drinks, dairy
products, egg products, soups and sauces, confectionery, chewing gum,
cosmetics, pharmaceuticals and other materials (e.g. biological cultures,
samples, etc.)
Method recognition: Novel method

Advantages

  • Only enzymatic kit available
  • Very cost effective
  • All reagents stable for > 2 years after preparation
  • Very rapid reaction
  • Mega-Calc™ software tool is available from our website for hassle-free raw data processing
  • Standard included
  • Suitable for manual, microplate and auto-analyser formats

 

 Q1. Should the pH of the sample be adjusted even for samples in acidic media?

The pH of the assay solution after the sample is added should be the same as that of the assay buffer that is supplied with the kit.
Low sample volumes (e.g. 0.1 mL) are not likely to affect the pH of the assay solution and therefore may not require pH adjustment.
Samples above 0.1 mL are more likely to affect the pH of the assay solution and therefore the pH of these samples should be adjusted as described in the data booklet, prior to addition to the assay.

Q2. Sometimes a negative absorbance change is obtained for the blank samples, is this normal? Should the real value (negative absorbance change) or “0” be used in the calculation of results?

Sometimes the addition of the last assay component can cause a small negative absorbance change in the blank samples due to a dilution effect and in such cases it is recommended that the real absorbance values be used in the calculation of results.

Q3. There is an issue with the performance of the kit; the results are not as expected.

If you suspect that the Megazyme test kit is not performing as expected such that expected results are not obtained please do the following:

  1. Ensure that you have tested the standard sample that is supplied with the Megazyme test kit.
  2. Send the results of the kit standard, blank samples and the results obtained for your sample, in the relevant MegaCalc spreadsheet (if available) to Megazyme (cs@megazyme.com). Where available the relevant MegaCalc spreadsheet can be downloaded from where the product appears on the Megazyme website.
  3. State the kit lot number being used (this is found on the outside of the kit box).
  4. State which assay format was used (refer to the relevant page in the kit booklet if necessary).
  5. State exact details of any modifications to the standard procedure that is provided by Megazyme.
  6. State the sample type and describe the sample preparation steps if applicable.

Q4. How can I work out how much sample to extract and what dilution of my sample should be used in the kit assay?

Where the amount of analyte in a liquid sample is unknown, it is recommended that a range of sample dilutions are prepared with the aim of obtaining an absorbance change in the assay that is within the linear range.
Where solid samples are analysed, the weight of sample per volume of water used for sample extraction/preparation can be altered to suit, as can the dilution of the extracted sample prior to the addition of the assay, as per liquid samples.

Q5. I have some doubts about the appearance/quality of a kit component what should be done?

If there are any concerns with any kit components, the first thing to do is to test the standard sample (control sample) that is supplied with the kit and ensure that the expected value (within the accepted variation) is obtained before testing any precious samples. This must be done using the procedure provided in the kit booklet without any modifications to the procedure. If there are still doubts about the results using the standard sample in the kit then send example results in the MegaCalc spread sheet to your product supplier (Megazyme or your local Megazyme distributor).

Q6. How much sample should be used for the clarification/extraction of my sample?

The volume/weight of sample and total volume of the extract can be modified to suit the sample. This will ultimately be dictated by the amount of analyte of interest in the sample and may require empirical determination. For low levels of analyte the sample:extract volume ratio can be increased (i.e. increase the sample and/or decrease the total extraction volume).

Alternatively, for samples with low concentrations of analyte, a larger sample volume can be added to the kit assay. When altering the sample volume adjust the distilled water volume added to the assay accordingly so that the total assay volume is not altered.

Q8. Can the test kit be used to measure biological fluids and what sample preparation method should be used?

The kit assay may work for biological fluids assuming that inositol is present above the limit of detection for the kit after any sample preparation (if required). Centrifugation of the samples and use of the supernatant directly in the kit assay (with appropriate dilution in distilled water) may be sufficient. However, if required a more stringent sample preparation method may be required and examples are provided at the following link:http://www.megazyme.com/docs/analytical-applications-downloads/biological_samples_111109.pdf?sfvrsn=2

The test kit has not been tested using biological fluids as samples because it is not marketed or registered as a medical device. This will therefore require your own validation.

Q9. Can the manual assay format be scaled down to a 96-well microplate format?

The majority of the Megazyme test kits are developed to work in cuvettes using the manual assay format, however the assay can be converted for use in a 96-well microplate format. To do this the assay volumes for the manual cuvette format are reduced by 10-fold. The calculation of results for the manual assay format uses a 1 cm path-length, however the path-length in the microplate is not 1 cm and therefore the MegaCalc spreadsheet or the calculation provided in the kit booklet for the manual format cannot be used for the micropalate format unless the microplate reader being used can.

There a 3 main methods for calculation of results using the microplate format:

  1. The easiest method is to use a microplate reader that has a path-length conversion capability (i.e. the microplater reader can detect the path-length of each well and convert the individual readings to a 1 cm path-length). This will allow values to be calculated using the MegaCalc calculation software which can be found where the product is located on the Megazyme website.
  2. Perform a standard curve of the analyte on each microplate that contains test samples and calculate the result of the test samples from the calibration curve (concentration of analyte versus absorbance).
  3. Perform a standard curve of the analyte in both the cuvette format (i.e. with a 1 cm path-length) and the 96-well microplate format and use these results to obtain a mean conversion factor between the cuvette values and the microplate values. Subsequent assays in the microplate format can then be converted from the calculated conversion factor.

Q10. Can the sensitivity of the kit assay be increased?

For samples with low concentrations of analyte the sample volume used in the kit assay can be increased to increase sensitivity. When doing this the water volume is adjusted to retain the same final assay volume. This is critical for the manual assay format because the assay volume and sample volume are used in the calculation of results.

Q11. When using this kit for quantitative analysis what level of accuracy and repeatability can be expected?

The test kit is extremely accurate – at Megazyme the quality control criteria for accuracy and repeatability is to be within 2% of the expected value using pure analytes.

However, the level of accuracy is obviously analyst and sample dependent.

Q12. Is it possible to add a larger volume then 2 μL of enzyme to the microplate assay? In some instances 2 μL can be difficult to pipette manually.

Yes, instead of adding 2 μL of enzyme suspension an alternative is to dilute the enzyme and add a larger volume to the microplate assay.

Dilute the assay buffer 10-fold with distilled water and use this as the diluent to dilute an aliquot of the enzyme suspension also by 10-fold. Instead of 2 μL, use 20 μL of the diluted enzyme in the microplate assay.

Q13. Must the minimum absorbance change for a sample always be at least 0.1?

No. The 0.1 change of absorbance is only a recommendation. The lowest acceptable change in absorbance can is dictated by the analyst and equipment (i.e. pipettes and spectrophotometer) and therefore can be can be determined by the user. With accurate pipetting, absorbance changes as low as 0.02 can be used accurately.
If a change in absorbance above 0.1 is required but cannot be achieved due to low concentrations of analyte in a sample, this can be overcome by using a larger sample volume in the assay to increase the absorbance change and thereby increase sensitivity of the assay. When doing this the increased volume of the sample should be subtracted from the distilled water volume that is added to the assay so that the total assay volume is unaltered. The increase sample volume should also be accounted for when calculating final results. 

Q14. Can the sensitivity of the kit assay be increased?

Yes. Samples with the lower concentrations of analyte will generate a lower absorbance change. For samples with low concentrations of analyte, a larger sample volume can be used in the assay to increase the absorbance change and thereby increase sensitivity of the assay. When doing this the increased volume of the sample should be subtracted from the distilled water volume that is added to the assay so that the total assay volume is unaltered. The increase sample volume should also be accounted for when calculating final results.