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34367-04-9

中文名称 人参皂苷RO
英文名称 GinsenosideRo
CAS 34367-04-9
分子式 C48H76O19
分子量 957.11
MOL 文件 34367-04-9.mol
更新日期 2024/04/22 13:36:53
34367-04-9 结构式 34367-04-9 结构式

基本信息

中文别名
竹节参苷V
竹节参皂苷V
人参皂苷RO
人参皂苷RO对照品,
人参皂苷RO(标准品)
人参皂苷RO(分析标准品)
人参皂苷RO、 竹节参苷V
人参皂苷RO/竹节参苷V 标准品
人参皂苷ROGINSENOSIDE RO
英文别名
PolysciasaponinP3
HericiuMsaponin S3
Chikusetusaponin V
ChikusetsusaponinV
Chikusetsusaponin 5
Ginseng Extract – Ginsenoside
28-(β-D-Glucopyranosyloxy)-28-oxoolean-12-en-3β-yl 2-O-β-D-glucopyranosyl-β-D-glucopyranosiduronic acid
3β-(2-O-β-D-Glucopyranosyl-β-D-glucopyranuronosyloxy)oleana-12-ene-28-oic acid 28-β-D-glucopyranosyl ester
28-(β-D-Glucopyranosyloxy)-28-oxo-5α-olean-12-en-3β-yl 2-O-β-D-glucopyranosyl-β-D-glucopyranosiduronic acid
β-D-Glucopyranosiduronic acid, (3β)-28-(β-D-glucopyranosyloxy)-28-oxoolean-12-en-3-yl2-O-β-D-glucopyranosyl-
所属类别
生物化工:提取物

物理化学性质

外观性状白色粉末,易溶于甲醇乙醇,来源于人参。
沸点1018.6±65.0 °C(Predicted)
密度1.14
储存条件Store at 2-8°C, protect from light
溶解度DMSO : 100 mg/mL (104.48 mM; Need ultrasonic)
酸度系数(pKa)2.76±0.70(Predicted)
形态粉末
颜色白色

安全数据

危险性符号(GHS)
GHS07
警示词警告
危险性描述H302
海关编码29389090

应用领域

用途1
用于含量测定/鉴定/药理实验等。
药理药效:人参主要具有大补元气,滋补强壮,安神益智,生津,复脉固脱等功效。
用途2
人参皂苷Ro是人参根茎的主要皂苷成分,有抗炎症、抗肝炎等生物活性。

图谱信息

人参皂苷RO价格(试剂级)
报价日期产品编号产品名称CAS号包装价格
2024/01/16S9103人参皂苷RO
Ginsenoside Ro
34367-04-91mg1204.38元

常见问题列表

生物活性
Ginsenoside Ro (Polysciasaponin P3; Chikusetsusaponin 5; Chikusetsusaponin V) 具有 Ca2+ 拮抗剂的抗血小板作用,IC50 为 155  μM。Ginsenoside Ro 降低 TXA2 产量,Ginsenoside Ro 还稍弱地降低 COX-1 和 TXAS 活性。
靶点

TXA 2

Ca 2+

体外研究

Ginsenoside Ro in Panax ginseng is a beneficial novel Ca 2+ -antagonistic compound and may prevent platelet aggregation-mediated thrombotic disease. Ginsenoside Ro dose-dependently reduces thrombin-stimulated platelet aggregation, and IC 50 is approximately 155 μM. Ginsenoside Ro inhibits TXA 2 production to abolish thrombin-induced platelet aggregation. Thromboxane A 2 (TXA 2 ) induces platelet aggregation and promotes thrombus formation. Ginsenoside Ro dose-dependently (50-300 μM) reduces the TXB 2 level that is induced by thrombin; Ginsenoside Ro (300 μM) inhibits the thrombin-mediated elevation in TXB 2 level by 94.9%. COX-1 activity in the absence of Ginsenoside Ro (negative control) is 2.3±0.1 nmol/mg protein. However, Ginsenoside Ro dose-dependently (50-300 μM) reduces its activity; at 300 μM, COX-1 activity is reduced by 26.4% of that of the negative control. TXA 2 synthase (TXAS) activity in the absence of Ginsenoside Ro (negative control) is 220.8±1.8 ng/mg protein/min. However, Ginsenoside Ro dose-dependently (50-300 μM) reduces its activity; at 300 μM, TXAS activity is reduced by 22.9% of that of the negative control. The inhibitory effect of Ginsenoside Ro (300 μM) on TXB 2 production (94.9%) is significantly higher than those on COX-1 (26.4%) and TXAS (22.9%) activities. To assess the toxicity of Ginsenoside Ro in Raw 264.7 cells, they are first treated with various concentrations (10 μM, 50 μM, 100 μM, and 200 μM) of Ginsenoside Ro for 24 h. Ginsenoside Ro exhibits no significant dose dependent toxicity. The effect of Ginsenoside Ro is next determined on cell viability and ROS levels, a marker of oxidative stress, following treatment with 1 μg/mL LPS. LPS reduces cell viability by ∼70% compared with nontreated controls. Pretreatment with 100 μM and 200 μM Ginsenoside Ro for 1 h prior to 1 μg/mL LPS incubation for 24 h leads to a significant increase in cell viability. The changes in ROS levels and NO production are consistent with the effects of Ginsenoside Ro on viability.

体内研究

Ginsenoside Ro dissolved in water is administrated by gavage to mice at doses of 25 and 250 mg/kg/day for 4 days before i.v. injection of HT29 in order to keep blood concentrations of Ginsenoside Ro above a certain level before HT29 i.v. injection followed by 40 days of oral administration of Ginsenoside Ro to the mice. After 38 days of treatment, the animals are euthanized, and the number of pulmonary metastatic nodules is counted in addition to evaluation of toxicity of Ginsenoside Ro and mouse pathology by HT29. Ginsenoside Ro (250 mg/kg/day) produces a significant decrease in the number of tumor nodules on the lung surface, yielding inhibition rates of 88% (P [4] .

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