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- 文献和实验
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- 保存条件:
常温
- 保质期:
根据瓶身LOT号查询
- 英文名:
Trizma® 马来酸盐
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
72200-76-1
- 规格:
50G
属性
方案
≥99.5% NaOH basis (anhydrous, titration)
质量水平
200
表单
crystalline powder
溶解性
water: 500 mg/mL, clear, colorless
SMILES字符串
NC(CO)(CO)CO.OC(=O)\C=C/C(O)=O
InChI
1S/C4H11NO3.C4H4O4/c5-4(1-6,2-7)3-8;5-3(6)1-2-4(7)8/h6-8H,1-3,5H2;1-2H,(H,5,6)(H,7,8)/b;2-1-
InChI key
HTMWOUBCEZXSHN-BTJKTKAUSA-N
应用
- 在痰液中对胞旋标本进行免疫细胞化学分析
- 核苷二磷酸酶检测前的脊髓切片孵育
- 作为胚胎干细胞碱性磷酸 (AP) 染色的组分
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文献和实验Midface and upper airway dysgenesis in FGFR2-related craniosynostosis involves multiple tissue-specific and cell cycle effects.
Midface dysgenesis is a feature of more than 200 genetic conditions in which upper airway anomalies frequently cause respiratory distress, but its etiology is poorly understood. Mouse models of Apert and Crouzon craniosynostosis syndromes exhibit midface dysgenesis similar to the human conditions. They carry activating mutations of Fgfr2, which is expressed in multiple craniofacial tissues during development. Magnetic resonance microscopy of three mouse models of Apert and Crouzon syndromes revealed decreased nasal passage volume in all models at birth. Histological analysis suggested overgrowth of the nasal cartilage in the two Apert syndrome mouse models. We used tissue-specific gene expression and transcriptome analysis to further dissect the structural, cellular and molecular alterations underlying midface and upper airway dysgenesis in Apert Fgfr2+/S252W mutants. Cartilage thickened progressively during embryogenesis because of increased chondrocyte proliferation in the presence of Fgf2 Oral epithelium expression of mutant Fgfr2, which resulted in a distinctive nasal septal fusion defect, and premature facial suture fusion contributed to the overall dysmorphology. Midface dysgenesis in Fgfr2-related craniosynostosis is a complex phenotype arising from the combined effects of aberrant signaling in multiple craniofacial tissues.
green快速染料标记1 × 104个TYK-nu细胞,96孔板放置4h,然后加入2 × 104个或5 × 104个T细胞和激活剂scDb(anti-CD3ε scFv,单链双特异性抗体形式)进行共培养。不断减少的绿色荧光信号,表明激活的T细胞具有显著的免疫杀伤作用。同时,通过Incucyte®系统的10×物镜连续拍摄120h,计算每孔中每mm2的gfp阳性对象数量,发现H2-scDb介导的细胞毒性同样通过TP53的破坏而减轻。 2. Nature:神经细胞吞噬及分化 应用领域:神经
采用UPC2/MS/MS分离利培酮的活性对映体代谢物并用于检测代谢稳定性
了从母体化合物到羟基代谢物的转化过程。 本方法被用于分析t在0、15、30、60、90和120 min时淬灭的温育样品,以监测从利培酮母体到9-羟基代谢物的转化过程。图2显示了一个示例进样,其中9-羟基代谢物的两个预期峰分别位于3.92和4.29 min处。然而,在4.48和4.76 min处还出现了另外两个峰,它们可能是文献报道的少量7-羟基利培酮代谢物。1 图1. 利培酮(上)和R/S 9-羟基利培酮(下)。 图1展示了采用沃特世(Waters®)Trefoil
蛋白表达系统在表达膜蛋白、有毒蛋白、二硫键蛋白、抗体片段等方面具有独特优势。由于可以使用线性模板,利用PCR方法就可以轻松实现在目的基因两侧加入需要的转录和翻译所需的因子,不需要繁琐的载体构建过程。线性模板的使用还可以实现蛋白的高通量合成和筛选。 ALiCE® Kit无细胞蛋白质表达试剂盒 (植物细胞裂解液) (Sigma货号:AL0103000) ALiCE®无细胞蛋白质表达试剂盒是一种独创的真核无细胞系统,可利用植物细胞裂解物在批量处理模式下将蛋白质产量提升到前所未有的3mg/mL。ALiCE®
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