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- 英文名:
Phytagel
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
71010-52-1
- 规格:
1KG
属性
产品线
BioReagent
质量水平
200
表单
powder
技术
cell culture | plant: suitable
应用
agriculture
一般描述
应用
- 拟南芥中根检测的培养基固化
- 作为农杆菌培养中固体Paul′s培养基的一种成分
- 冬青属组织培养中根诱导培养基的一种组分
生化/生理作用
制备说明
其他说明
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文献和实验A Tobacco Syringe Agroinfiltration-Based Method for a Phytohormone Transporter Activity Assay Using Endogenous Substrates.
Phytohormones are a group of small chemical molecules that play vital roles in plant development, metabolism, and stress responses. Phytohormones often have distinct biosynthesis and signaling perception sites, requiring long- or short-distance transportation. Unlike biosynthesis and signal transduction, phytohormone transport across cells and organs is poorly understood. The transporter activity assay is a bottleneck for the functional characterization of novel phytohormone transporters. In the present study, we report a tobacco syringe agroinfiltration and liquid chromatography tandem mass spectrometry (TSAL)-based method for performing a phytohormone transporter activity assay using endogenous hormones present in tobacco (Nicotiana benthamiana) leaves. A transporter activity assay using this method does not require isotope-labeled substrates and can be conveniently performed for screening multiple substrates by using endogenous hormones in tobacco leaves. The transporter activities of three known hormone transporters, namely AtABCG25 for abscisic acid, AtABCG16 for jasmonic acid, and AtPUP14 for cytokinin, were all successfully validated using this method. Using this method, cytokinins were found to be the preferred substrates of an unknown maize (Zea mays) transporter ZmABCG43. ZmABCG43 transporter activities toward cytokinins were confirmed in a cytokinin long-distance transport mutant atabcg14 through gene complementation. Thus, the TSAL method has the potential to be used for basic substrate characterization of novel phytohormone transporters or for the screening of novel transporters for a specific phytohormone on a large scale.
Replication timing by density transfer
, leu2-3,112, ura3-52, his6 in an A364A background. I aim for about 32 x 106 cells per time point. That gives enough DNA for at least 3 blots, leaving enough leeway for errors. 2. When the cell density is 2 x 106 cells/ml (OD660 ~ 0.16
Detection of apoptotic process in situ using immunocytochemical and TUNEL assays
in individual apoptotic cells by the in situ terminal deoxynucleotidyl transferase and nick translation assays. Cancer Res . 52: 1945. 3. Gorczyca, W.,Tuziak,T., Kram, A., Melamed, M.R., Darzynkiewicz, Z. 1994. Detection of apoptosis-associated DNA strand
Purpose: Mini-prep method for lambda phage DNA purification from lysates. Time required: 4 hours once the lysate is in handSpecial supplies required: BioRad Econo Columns (Cat.# 731-1550) Whatman DE-52 (Fisher Cat.#05-720-5)
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