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- 文献和实验
- 技术资料
- 保存条件:
常温
- 保质期:
根据瓶身LOT号查询
- 英文名:
2-Hydroxyethyl cellulose
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
9004-62-0
- 规格:
250G
属性
表单
powder
自燃温度
725 °F
分子量
average Mv ~90,000
标记范围
2.5 mol per mol cellulose (M.S.)
粘度
100-180 cP(lit.)
密度
0.6 g/mL at 25 °C (lit.)
SMILES字符串
O1C(C(C(C(C1CO)OC)O)OCCO)OC2C(OC(C(C2O)O)OC4C(OC(C(C4O)O)C)CO)COC3OC(C(C(C3O)O)OC)CO
InChI
1S/C29H52O21/c1-10-15(34)16(35)24(13(8-33)45-10)49-28-20(39)18(37)25(50-29-26(43-5-4-30)21(40)23(42-3)12(7-32)47-29)14(48-28)9-44-27-19(38)17(36)22(41-2)11(6-31)46-27/h10-40H,4-9H2,1-3H3
InChI key
CWSZBVAUYPTXTG-UHFFFAOYSA-N
一般描述
应用
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文献和实验Capacitively coupled contactless conductivity detection for microfluidic capillary isoelectric focusing.
We report capacitively coupled contactless conductivity detection (C4D) of proteins separated by microfluidic capillary isoelectric focusing (μCIEF). To elucidate the evolution of negative conductivity peaks during focusing and seek IEF conditions for sensitive conductivity detection, numerical simulation was performed using a model protein GFP (green fluorescence protein) and hypothetical carrier ampholytes (CAs). C4D was successfully applied to the μCIEF by optimizing assay conditions using a simple and effective pressure-mobilization approach. The conductivity and fluorescence signals of a focused GFP band were co-detected, confirming that the obtained negative C4D peak could be attributed to the actual protein, not the non-uniform background conductivity profile of the focused CAs. GFP concentrations of 10 nM-30 μM was quantified with a detection limit of 10 nM. Finally, the resolving power was analyzed by separating a mixture of R-phycoerythrin (pI 5.01), GFP-F64L (pI 5.48), and RK-GFP (pI 6.02). The conductivities of the three separated fluorescence proteins were measured with average separation resolution of 2.06. We expect the newly developed label-free μCIEF-C4D technique to be widely adopted as a portable, electronics-only protein-analysis tool.
0:05 无有机溶剂和醋酸时蛋白质凝胶的考马斯亮蓝G-250染色法5 0:21 内容订阅21 1:02 内容简介62 1:34 配制考马斯亮蓝染色溶液94 2:38 SDS-PAGE电泳158 4:26 凝胶染色266 6:38 代表性实验结果398 7:19 结论439 无有机溶剂和醋酸时蛋白质凝胶的考马斯亮蓝G-250染色法本视频来源于网络,如有异议请联系我们,我们将在5个工作日内作出处理。
实验62 脱落酸(ABA)放射免疫测定 原理 ABA放射免疫测定(radioimmunoassay, RIA)是一种分子相同的标记ABA(*Ag)和非标记ABA(Ag)与另一种浓度有限的专一性抗ABA抗体(Ab)进行的竞争性抑制反应: 当反应体系中*Ag和Ab量保持恒定,并且*Ag量>Ab量(*Ag: Ab100: 35)时,加入的Ag量越多,则*Ag被稀释的程度也就越
) (store at 4deg.C). IPTG (isopropyl b-D-thiogalactopyranoside):25 mg/ml IPTG in double distilled water 250 mg IPTG (Sigma I-5502) ddH2 O to 10 ml (aliquot and store at -20℃) 1 M isocitrate (sodium salt-dihydrate) : 29.41 g Na3isocitrate-2H
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