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作 者:艾合买提.买买提 买合布白.阿不都热依木 艾克白尔.买买提 阿布都热依木.阿布都克日木
机构地区:[1]新疆维吾尔自治区维吾尔医医院科研科,新疆乌鲁木齐830049
出 处:《药学进展》2010年第5期228-230,共3页Progress in Pharmaceutical Sciences
基 金:"十一五"国家科技支撑计划(2007BAI48B06)
摘 要:目的:建立HPLC法测定玫瑰花瓣中槲皮素含量,并对两个产地玫瑰花瓣中槲皮素含量进行比较。方法:色谱柱:Symmetry Shield RP18(150mm×4.6mm,5μm);柱温:25℃;检测波长:368nm;流速:1.0mL.min-1;流动相:甲醇-0.4%磷酸(60∶40);进样量:10μL。结果:槲皮素的平均回收率为98.4%(RSD=1.78%,n=9);和田玫瑰花瓣提取物水解样中槲皮素含量为(3.05±0.090)mg.g-1(RSD=2.95%,n=3),未水解样中槲皮素含量为(0.405±0.013)mg.g-1(RSD=3.21%,n=3);昌吉玫瑰花瓣提取物水解样中槲皮素含量为(1.841±0.013)mg.g-1(RSD=1.84%,n=3),未水解样中槲皮素含量为(0.225±0.007)mg.g-1(RSD=3.11%,n=3),和田玫瑰花瓣中槲皮素含量高于昌吉玫瑰花瓣。结论:该方法简便、快速、准确,可用于玫瑰花瓣中槲皮素含量测定及药材质量控制。Objective: To establish a HPLC method for the determination of quercetin in Rosa rugosa petal and to compare the contents of quercetin in Rosa rugosa from two sources. Methods: The determina- tion was performed on a Symmetry Shield RP18( 150 mm ×4.6 mm, 5 μm), and methanol-0. 4% phosphoric acid (60 : 40) were used as mobile phase at a column temperature of 25 ℃, at detection wave- length of 368 nm, and with a flow rate of 1.0 mL.min ^-1 and an injection volume of 10 μL. Results: The average recovery of quercetin was 98.4% ( RSD = 1.78%, n = 9). The contents of quercetin in the hydrolysis and un-hydrolysis samples from Hotan's Rosa rugosa petal extract were (3.05 ± 0. 090) mg .g^-1 ( RSD = 2. 95%, n = 3) and ( 0. 405 ± 0. 013) mg·g^- 1 ( RSD = 3.21%, n = 3), respectively, and those from Changji's Rosa rugosa petal extract were ( 1. 841 ± 0. 013) mg-g-1 ( RSD = 1.84%, n = 3) and (0. 225 ± 0. 007) mg. g^-1 ( RSD = 3.11%, n = 3), respectively. The contents of quercetin in the samples from Hotan were higher than those from Changji. Conclusion: This method is simple, rapid, accurate and reliable for the determination of quercetin in Rosa rugosa petal and also for the quality control of the raw material.
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