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- 详细信息
- 文献和实验
- 技术资料
- 保存条件:
2-8°C
- 保质期:
根据瓶身LOT号查询
- 英文名:
2-Deoxy-D-glucose
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
154-17-6
- 规格:
1G
属性
生物来源
synthetic
质量水平
200
方案
≥98% (GC)
表单
crystalline
技术
gas chromatography (GC): suitable
inhibition assay: suitable
颜色
white to off-white
mp
146-147 °C (lit.)
溶解性
H2O: 0.250 g/5mL
应用
clinical research
life science and biopharma
metabolomics
储存温度
2-8°C
SMILES字符串
OC[C@@H](O)[C@@H](O)[C@H](O)CC=O
InChI
1S/C6H12O5/c7-2-1-4(9)6(11)5(10)3-8/h2,4-6,8-11H,1,3H2/t4-,5-,6+/m1/s1
InChI key
VRYALKFFQXWPIH-PBXRRBTRSA-N
一般描述
应用
生化/生理作用
特点和优势
- 高纯度化合物适用于各种研究应用
包装
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文献和实验Defective glucose metabolism in polycystic kidney disease identifies a new therapeutic strategy.
Autosomal dominant polycystic kidney disease (ADPKD) is a common genetic disorder characterized by bilateral renal cyst formation. Recent identification of signaling cascades deregulated in ADPKD has led to the initiation of several clinical trials, but an approved therapy is still lacking. Using a metabolomic approach, we identify a pathogenic pathway in this disease that can be safely targeted for therapy. We show that mutation of PKD1 results in enhanced glycolysis in cells in a mouse model of PKD and in kidneys from humans with ADPKD. Glucose deprivation resulted in lower proliferation and higher apoptotic rates in PKD1-mutant cells than in nondeprived cells. Notably, two distinct PKD mouse models treated with 2-deoxyglucose (2DG), to inhibit glycolysis, had lower kidney weight, volume, cystic index and proliferation rates as compared to nontreated mice. These metabolic alterations depend on the extracellular signal-related kinase (ERK) pathway acting in a dual manner by inhibiting the liver kinase B1 (LKB1)-AMP-activated protein kinase (AMPK) axis on the one hand while activating the mTOR complex 1 (mTORC1)-glycolytic cascade on the other. Enhanced metabolic rates further inhibit AMPK. Forced activation of AMPK acts in a negative feedback loop, restoring normal ERK activity. Taken together, these data indicate that defective glucose metabolism is intimately involved in the pathobiology of ADPKD. Our findings provide a strong rationale for a new therapeutic strategy using existing drugs, either individually or in combination.
:Formerly listed as Type III 溶解性:溶于水,参考浓度2mg/ml 储存条件:2-8℃ From Sigma D1626 Salmon DNA 的配制: 组份浓度10 mg/ml Salmon DNA ;配制量约100 ml 配制方法: 1. 称取鲑鱼精DNA 2 g置于500 ml烧杯中,加入约200 ml的TE Buffer。 2. 用磁力搅拌器室温搅拌2~4小时
Th17 Polarization of Mouse CD4 Cells
-dibutyrate)[Details: Sigma, cat.#P1269] FICZ (6-formylindolo[3,2-b]carbazole)[Details: Life Sciences, cat. #BML-GR206-0100] 实验步骤 1. Isolation of CD4 cells from lymph nodes 1) Harvest lymph nodes (superfical cervical
乙酰基转移酶基因(bar),作为选择标记,该基因由花椰菜病毒启动子(CaMV35S ) 驱动,以农杆菌胭脂氨酸合成酶基因(nos ) 的 3' 非编码区为终止子。胁迫抗性基因来源于大麦胚胎发生后期的富集蛋白基因(Shva1) ,由水稻肌动蛋白 Act1 的启动子驱动,以马铃薯蛋白水解酶抑制子II ( pin ll ) 的 3' 非编码区为终止子( 图 10.1) 。 (2) pAct1-D:含有由 Act1 启动子驱动并利用 nos 终止子的大肠杆菌 β-葡萄糖醛酸酶基因(gus) ( 图
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