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Studies on Chromatographic Fingerprint and Fingerprinting Profile-Efficacy Relationship of Saxifraga stolonifera Meerb.

机译:虎耳草的色谱指纹图谱和指纹图谱-功效关系的研究。

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摘要

This work investigated the spectrum-effect relationships between high performance liquid chromatography (HPLC) fingerprints and the anti-benign prostatic hyperplasia activities of aqueous extracts from Saxifraga stolonifera. The fingerprints of S. stolonifera from various sources were established by HPLC and evaluated by similarity analysis (SA), hierarchical clustering analysis (HCA) and principal component analysis (PCA). Nine samples were obtained from these 24 batches of different origins, according to the results of SA, HCA and the common chromatographic peaks area. A testosterone-induced mouse model of benign prostatic hyperplasia (BPH) was used to establish the anti-benign prostatic hyperplasia activities of these nine S. stolonifera samples. The model was evaluated by analyzing prostatic index (PI), serum acid phosphatase (ACP) activity, concentrations of serum dihydrotestosterone (DHT), prostatic acid phosphatase (PACP) and type II 5α-reductase (SRD5A2). The spectrum-effect relationships between HPLC fingerprints and anti-benign prostatic hyperplasia activities were investigated using Grey Correlation Analysis (GRA) and partial least squares regression (PLSR). The results showed that a close correlation existed between the fingerprints and anti-benign prostatic hyperplasia activities, and peak 14 (chlorogenic acid), peak 17 (quercetin 5-O-β-d-glucopyranoside) and peak 18 (quercetin 3-O-β-l-rhamno-pyranoside) in the HPLC fingerprints might be the main active components against anti-benign prostatic hyperplasia. This work provides a general model for the study of spectrum-effect relationships of S. stolonifera by combing HPLC fingerprints with a testosterone-induced mouse model of BPH, which can be employed to discover the principle components of anti-benign prostatic hyperplasia bioactivity.
机译:这项工作调查了高效液相色谱(HPLC)指纹图谱和虎耳草水提取物的抗良性前列腺增生活性之间的光谱效应关系。通过HPLC建立了来自多种来源的S. stolonifera的指纹,并通过相似性分析(SA),层次聚类分析(HCA)和主成分分析(PCA)进行了评估。根据SA,HCA和共同色谱峰面积的结果,从这24个批次的不同来源中获得了9个样品。使用睾丸激素诱导的良性前列腺增生(BPH)小鼠模型来建立这9个stolonifera样品的抗良性前列腺增生活性。通过分析前列腺指数(PI),血清酸性磷酸酶(ACP)活性,血清二氢睾丸激素(DHT),前列腺酸磷酸酶(PACP)和II型5α-还原酶(SRD5A2)评估模型。使用灰色相关分析(GRA)和偏最小二乘回归(PLSR)研究了HPLC指纹图谱与抗良性前列腺增生活性之间的光谱效应关系。结果表明,指纹图谱与抗良性前列腺增生活性之间存在密切相关性,峰14(绿原酸),峰17(槲皮素5-O-β-d-吡喃葡萄糖苷)和峰18(槲皮素3-O-) HPLC指纹图中的β-1-鼠李糖-吡喃糖苷可能是抗良性前列腺增生的主要活性成分。这项工作通过结合HPLC指纹图谱和睾丸激素诱导的BPH小鼠模型,为研究S. stolonifera的光谱效应关系提供了一个通用模型,该模型可用于发现抗良性前列腺增生生物活性的主要成分。

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