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当前位置: 首页 > 产品中心 > Immunostain_staining_kit > 生物测定系统/酶染色与贸易;过氧化氢酶检测试剂盒/100次检测/ECAT-100
商品详细生物测定系统/酶染色与贸易;过氧化氢酶检测试剂盒/100次检测/ECAT-100
生物测定系统/酶染色与贸易;过氧化氢酶检测试剂盒/100次检测/ECAT-100
生物测定系统/酶染色与贸易;过氧化氢酶检测试剂盒/100次检测/ECAT-100
商品编号: ECAT-100
品牌: bioassaysys
市场价: ¥5580.00
美元价: 2790.00
产地: 美国(厂家直采)
公司:
产品分类: 免疫组化染色试剂盒
公司分类: Immunostain_staining_kit
联系Q Q: 3392242852
电话号码: 4000-520-616
电子邮箱: info@ebiomall.com
商品介绍

EnzyChrom™ Catalase Assay Kit

EnzyChrom™ Catalase Assay Kit Catalog No: ECAT-100
Price: $279 Qty:
For orders of 10 or more kits, please call +1-510-782-9988x1 oremail us for best pricing and/or bulk order. Shipping: On Ice Shipment: Fedex ServiceDelivery: 1-2 days (US), 3-6 days (Intl) Storage: -20°C
Catalase Assay Kit
  • Product Overview
  • Product FAQ
  • Product Citations
  • Assay Service
ProtocolSDS

Application

  • For quantitative determination of catalase activity and evaluation of drug effects on catalase activity.

Key Features

  • Sensitive and accurate. Use 10 μL sample. Linear detection range 0.2 to 5 U/L catalase activity.
  • Simple and Convenient. The procedure involves adding a Substrate to sample, incubation for 30 min, followed by a Detection Reagent and reading the optical density or fluorescence intensity.

Method

  • OD570nm, or FL530/585nm

Samples

  • Serum, plasma, urine, saliva, cell culture etc

Species

  • All

Size

  • 100 tests

Detection Limit

  • 0.2 U/L

Shelf Life

  • 6 months

More Details

  • CATALASE (EC 1.11.1.6), is an ubiquitous antioxidant enzyme that catalyzes the decomposition of hydrogen peroxide (H2O2) to water and oxygen. By preventing excessive H2O2 build up, catalase allows important cellular processes which produce H2O2 as a byproduct to occur safely. Deficiency in catalase activity has been associated with grey hair and peroxisomal disorder acatalasia. Simple, direct and high-throughput assays for catalase activity find wide applications. BioAssay Systems improved assay directly measures catalase degradation of H2O2 using a redox dye. The change in color intensity at 570nm or fluorescence intensity (λex/em = 530/585nm) is directly proportional to the catalase activity in the sample.

Regarding the technique used in the DPOD-100 peroxidase assay and the ECAT-100 catalase assay that seems to be really similar, how will we be sure that one of them will measure the catalase activity and the other the peroxidase?

The DPOD assay measures the conversion of the dye reagent and hydrogen peroxide, which are provided in large excess as substrates for cellular peroxidases. Endogenous catalase activity does not interfere with the assay, because it does not react with the dye reagent, hydrogen peroxide is in large excess, and the reaction is short (10 minutes), leaving the H2O2 concentration practically unchanged.The ECAT assays measures catalase activity by first incubating much lower concentrations of hydrogen peroxide with the samples for 30 minutes. Then the decrease in hydrogen peroxide is measured by adding the dye reagent and HRP in excess.

You will have 100 µL of each standard when you have pipetted all solutions for the standard curve. How stable are the 100 µl standards? Can they be used the next day to make another standard curve or can the values from the already made standard curve be used when you have other samples the next day?

The H2O2 standards are stable for an hour. Therefore assays should be run as soon as possible with the samples and standards. It is recommended that customers run standard curve in each experiment.For more detailed product information and questions, please feel free to Contact Us. Or for more general information regarding our assays, please refer to our General Questions.
Lin, Ting-An, et al (2019). Red Quinoa Bran Extracts Protects against Carbon Tetrachloride-Induced Liver Injury and Fibrosis in Mice via Activation of Antioxidative Enzyme Systems and Blocking TGF-beta1 Pathway. Nutrients 11.2: 395. Assay: Catalase in mice liver tissue. Cueno, Marni E., and Kuniyasu Ochiai (2018). Gingival periodontal disease (PD) level-butyric acid affects the systemic blood and brain organ: insights into the systemic inflammation of periodontal disease. Frontiers in immunology 9:1158. Assay: Catalase in rat blood cytosol. Kang, Changwoo, et al (2018). Therapeutic effect of ascorbic acid on dapsone-induced methemoglobinemia in rats. Clinical and experimental emergency medicine 5.3: 192. Assay: Catalase in rat plasma. Salvatori, Ornella, et al (2018). Candida albicans Ras1 inactivation increases resistance to phagosomal killing by human neutrophils. Infection and immunity 86.12: e00685-18. Assay: Catalase in Candida albicans cells. Camini, Fernanda Caetano, et al (2017). Oxidative stress in Mayaro virus infection. Virus research 236: 1-8. Assay: Catalase in human cells. Kang, Hyeon Hui, et al (2017). Chronic intermittent hypoxia induces liver fibrosis in mice with diet-induced obesity via TLR4/MyD88/MAPK/NF-kB signaling pathways. Biochemical and biophysical research communications 490.2: 349-355. Assay: Catalase in mice tissues. Kook, Sung-Ho, et al (2017). Dietary hydroxycinnamates prevent oxidative damages to liver, spleen, and bone marrow cells in irradiation-exposed mice. Food science and biotechnology 26.1: 279-285. Assay: Catalase in mice tissues. Oliveira, C. S., et al (2017). Moderate aerobic exercise on the recovery phase of gentamicin-induced acute kidney injury in rats. Life sciences 169: 37-42. Assay: Catalase in rat tissues. Pradhan, Arnab, et al (2017). Elevated catalase expression in a fungal pathogen is a double-edged sword of iron. PLoS pathogens 13.5: e1006405. Assay: Catalase in C. albicans cells. Cueno ME (2013). Orally supplemented catechin increases heme amounts and catalase activities in rat heart blood mitochondria: a comparison between middle-aged and young rats. Exp Gerontol. 48(11):1319-22. Assay: Catalase in rat blood mitochondria. Chiu CC et al (2012). Beneficial Effects of Ocimum gratissimum Aqueous Extract on rats with CCl(4)-Induced Acute Liver Injury. Evid Based Complement Alternat Med 2012:736752. Assay: Catalase in rat serum. Hadzi-Petrushev N et al (2012). L-2-oxothiazolidine-4-carboxylate influence on age- and heat exposure-dependent peroxidation in rat"s liver and kidney. J Therm Biol 37(5):361-365. Assay: Catalase in rat Kidney. Hadzi-Petrushev N et al (2012). L-2-oxothiazolidine-4-carboxylate influence on age- and heat exposure-dependent peroxidation in rat"s liver and kidney. J Therm Biol 37(5):361-365. Assay: Catalase in rat Kidney.Zhu T et al (2012) Effects of the iron-chelating agent deferoxamine on triethylene glycol dimethacrylate, 2-hydroxylethyl methacrylate, hydrogen peroxide-induced cytotoxicity. J Biomed Mater Res B Appl Biomater 100(1):197-205. Assay: Catalase in human dental pulp cells. Hadzi-Petrushev N et al (2011) L-2-oxothiazolidine-4-carboxylate influence on age- and heat exposure-dependent redox changes in rat"s blood plasma. J Physiol Sci 61(5):437-442. Assay: Catalase in rat plasma. Labib, HM, et al (2010). The Role of Oxidative Stress Markers and Nitric Oxide Levels in the Pathogenesis of Glaucoma. Austr. J. Basic and Applied Sci 4(8): 3553-3558. Assay: Catalase in human blood. To find more recent publications, pleaseclick here.
If you or your labs do not have the equipment or scientists necessary to run this assay, BioAssay Systems can perform the service for you.Simply send us your samples:- Fast turnaround - Quality data - Low costPlease email or call 1-510-782-9988 x 2 to request assay service.
品牌介绍
BioAssay Systems位于加州北部,是一家专注于提供高质量试剂盒的生物技术公司,试剂盒种类广泛、使用简便、操作简单、快速且性能优越,用户不需花额外的时间来作调适测试。BioAssay Systems产品具有快速、简单、高通量(可用于HTS药物筛选)、灵敏(特别适合小鼠样品) 、准确性高和低干扰等主要特征,且采用发光、生物发光、化学发光、荧光等非放射性的检测技术,安全无害可靠。