Optimization of conditions for supercritical fluid extraction of flavonoids from hops (Humulus lupulus L.)

Waste hops are good sources of flavonoids. Extraction of flavonoids from waste hops (SC-CO2 extracted hops) using supercritical fluids technology was investigated. Various temperatures, pressures and concentrations of ethanol (modifier) and the ratio (w/w) of solvent to material were tested in this study. The results of single factor and orthogonal experiments showed that at 50 °C, 25 MPa, the ratio of solvent to material (50%), ethanol concentration (80%) resulted in maximum extraction yield fla- vonoids (7.8 mg/g). HPLC-MS analysis of the extracts indicated that flavonoids obtained were xanthohumol, the principal prenylflavonoid in hops.

Humulus lupulus L. Extract Prevents Ovariectomy-Induced Osteoporosis in Mice and Regulates Activities of Osteoblasts and Osteoclasts

Objective:To systematically evaluate the protective effects of Humulus lupulus L.extract(HLE)on osteoporosis mice.Methods:In vivo experiment,a total of 3512-week-old female ICR mice were equally divided into 5 groups:the sham control group(sham);the ovariectomy with vehicle group(OVX);the OVX with estradiol valerate[EV,0.2 mg/(kg·d)];the OVX with low-or high-dose HLE groups[HLE,1 g/(kg·d)and 3 g/(kg·d)],7 in each group.Treatment began 1 week after the ovariectomized surgery and lasted for 12 weeks.Bone mass and trabecular bone mircoarchitecture were evaluated by micro computed tomography,and bone turnover markers in serum were evaluated using enzyme-linked immunosorbent assay(ELISA)kits.In vitro experiment,osteoblasts and osteoclasts were treated with HLE at doses of 0,4,20 and 100μg/mL.Biomarkers for bone formation in osteoblasts and bone resorption in osteoclasts were analyzed.Results:Compared with the OVX group,HLE exerted bone protective effects by the increase of estradiol(P<0.05),the improvement of cancellous bone structure,bone mineral density(P<0.01)and the reduction of serum alkaline phosphatase(ALP),tartrate resistant acid phosphatase(TRAP),bone gla-protein,c-terminal telopeptides of typeⅠcollagen(CTX-Ⅰ)and deoxypyridinoline levels(P<0.01 for all).In vitro experiment,compared with the control group,HLE at 20μg/mL promoted the cell proliferation(P<0.01),and increased the expression of bone morphogenetic protein-2 and osteopontin levels in osteoblasts(both P<0.05).HLE at 100μg/mL increased the osteoblastic ALP activities,and HLE at all dose enhanced the extracellular matrix mineralization(both P<0.01).Furthermore,compared with the control group,HLE at 20μg/m L and 100μg/m L inhibited osteoclastic TRAP activity(P<0.01),and reduced the expression of matrix metalloproteinase-9 and cathepsin K(both P<0.05).Conclusion:HLE may protect against bone loss,and have potentials in the treatment of osteoporosis.

啤酒花(Humulus lupulus)茎尖培养快速繁殖的研究

对啤酒花茎尖培养生比分化培养条件、生根方法及试管苗移栽作了研究。表明茎尖作外植体材料时,适合于生长和分化的培养基组合为 MS+BA10^(-5)mol·L^(-1)+2,4-D^(-6)mol·L^(-1)+GA_310^(-6)mol·L^(-1)+ 葡萄糖30 g·L^(-1)+琼脂0.94%,P^H5.1。培养周期为3周。增殖系数5～7,分化株率95%,平均嫩茎高度1.7cm。适于生根的培养基组合为 KM+BA10^(-7)mol·L^(-1)+IBA10^(-8)mol·L^(-1)+葡萄糖20～30g·L^(-1)+琼脂0.85%,GA_310^(-6)mol·L^(-1)或不加,pH5.4。生根培养时用 IBA10^(-3) mol·L^(-1)预处理小插条基部对生根有促进作用。小插条用 IBA(10^(-4)～10^(-5)mol·L^(-1))速沾5s,能在试管外扦插生根,生根株率为68%,生根苗能顺利成活和生长。

Impact of Hydroalcoholic Extract of Humulus Lupulus L. on Sperm Quality, Reproductive Organs and Hormones in Male Rats

Objective: To investigate the impact of Humulus Lupulus L. hydroalcoholic extract on the body weights, reproductive organs, sperm quality and hormone levels in male rats. Methods: By simple random sampling method, seventy male Sprague-Dawley rats were randomly assigned to 7 groups including control group [distilled water, 1 mL/(kg·d)], Tween 80 group [25% Tween 80 solution, 1 mL/(kg·d)], olive oil group [olive oil, 1 mL/(kg·d)], diethyl stilbestrol(DES) group [DES, 100 μg/(kg·body weight)], H50, H150 and H450 [50, 150 and 400 mg/(kg·d) of Humulus Lupulus L extract, respectively]. The administration was performed via gavage once daily for 7 weeks. Body and reproductive organs weights including testes, seminal vesicles, epididymis and prostate were weighted and epididymal sperm quality were determined by digital balance. Blood samples were collected and serum free testosterone(T), luteinizing hormone(LH), follicle-stimulating hormone(FSH), and estrogen(E2) levels were measured by rat specific enzyme-linked immunosorbent assay. Results: The percentage increase in mean body weights of rats in the DES and H50, H150 and H450 groups decreased significantly compared to olive oil and Tween 80 groups(all P<0.05). The weights of seminal vesicle, epididymis and testes in rats receiving H50 were significantly higher than the control group(P<0.05 or P<0.01). The sperm count in the rats receiving H50 was significantly lower than the control group(P<0.05). The sperm motile characteristics of the rats receiving hydroalcoholic extract and DES were significantly lower than those of the control or rats receiving vehicles(all P<0.05). In H50, H150, H450 and DES groups, T and LH levels were decreased, and E2 was significantly increased compared to the control(P<0.05 or P<0.01). The FSH level did not change in all groups(P>0.05). Conclusion: Humulus Lupulus L. extract significantly increased the seminal vesicle and testes weights and reduced the sperm motility.

A Novel Prenylchalcone from Humulus lupulus

s: From hops of Humulus lupulus, a novel prenylchalcone was isolated, which showed inhibition against BGC-823 cells. The structure was elucidated as 5'-(2''-hydroxyisopropyl-)- dihydrofurano-[2', 3'-B]-4, 4'-dihydroxy-6'-methoxychalcone, by HRFABMS and NMR spectra.

葎草DNA的提取及AFLP标记反应体系的建立

本文对CTAB法、改良CTAB法和SDS法提取雌雄异株植物葎草(Humulus scandensL.)基因组的方法进行了比较分析,并在此基础上对影响葎草AFLP扩增的关键因素模板浓度、酶切时间、选择性扩增模板浓度进行了优化。结果表明,改良的CTAB法更适合葎草基因组DNA的提取;同时利用AFLP分子标记技术,采用EcoI-MseⅠ酶切组合,共筛选27对引物组合,确定了适用于葎草AFLP反应的最佳酶切连接、预扩和选扩体系。同时发现2对引物组合E-ACG+M-CTA和E-AAC+M-CAC共扩增出5条雌雄性别特异条带。

黄腐酚对高尿酸血症大鼠血尿酸水平及骨代谢的调控作用

目的考察黄腐酚(XAN)对高尿酸血症(HUA)大鼠的降血尿酸(UA)及调控骨代谢活性作用。方法将48只雄性Wistar大鼠随机分为6组(n=8):空白组,模型组,别嘌醇(ALLO)组,黄腐酚低剂量(XAN-L)组、中剂量(XAN-M)组、高剂量(XAN-H)组。采用氧嗪酸钾(200 mg·kg^(-1)·d^(-1))与次黄嘌呤(250 mg·kg^(-1)·d^(-1))联用法建立HUA模型。造模2 h后,各药物组分别给予相应药物混悬液(ALLO 20 mg·kg^(-1)·d^(-1),XAN5 mg·kg^(-1)·d^(-1),XAN 15 mg·kg^(-1)·d^(-1),XAN 45 mg·kg^(-1)·d^(-1)),灌胃干预14 d。分别于第3、7、10、14天进行眼眶取血,检测血清中UA、肌酐(CRE)、尿素氮(BUN)水平及黄嘌呤氧化酶(XOD)活性。实验结束测定碱性磷酸酶(ALP)活性,以及骨代谢相关蛋白Runt相关转录因子2(Runx2)、组织蛋白酶K(CTSK)、核因子κB受体活化因子配体(RANKL)和护骨因子(OPG)水平,并对RANKL/OPG比值进行分析。结果与空白组相比,第3、7、10、14天模型组大鼠血清UA水平升高(均P<0.01),表明大鼠HUA模型成功构建。与模型组相比,XAN-M、XAN-H可有效降低急、慢性HUA大鼠血清UA水平(均P<0.01)、抑制XOD活性(均P<0.01)、改善肾功能指标CRE(均P<0.01)和BUN(均P<0.05)。XAN-L虽未明显降低急性HUA大鼠的血清UA水平,但可有效降低XOD活性(P<0.01),并改善其肾功能指标CRE(P<0.01)和BUN(P<0.05);而对于慢性HUA大鼠,其能够有效降低血清UA水平(均P<0.01),却无明显肾保护作用。各剂量组XAN还可不同程度增强HUA大鼠的ALP活性(均P<0.01)、上调Runx2表达(XAN-L组除外,均P<0.01)、下调CTSK的表达(均P<0.01)、抑制RANKL分泌(均P<0.01)、促进OPG的表达(仅XAN-H组,P<0.01)、纠正RANKL/OPG的比值(均P<0.05)。结论XAN具有降低HUA大鼠血UA水平的作用,这可能与其抑制XOD活性以减少UA生成及保护肾功能以加强UA排泄有关;XAN还具有促进骨形成、抑制骨破坏,有效调控骨代谢的作用,这可能与其通过RANKL/OPG信号通路抑制破骨细胞分化有关。

啤酒花中单宁的提取及其对铜片在NaCl溶液中的缓蚀作用研究

在单因素试验的基础上,采用响应面分析法优化啤酒花中单宁的提取工艺,并对单宁在Na Cl溶液中对铜片的缓蚀作用进行考察。结果表明,啤酒花单宁提取最佳工艺条件为:提取时间152 min,提取温度48℃,料液比1∶26(g/m L)。在此条件下,啤酒花中单宁的提取率为1.340%,与理论值相差0.063%。静态失重法结果表明,在缓蚀温度为30℃、啤酒花单宁提取液体积为25 m L时,啤酒花单宁具有良好的缓蚀性能,缓蚀效率达到88.31%;通过动电位极化曲线测试研究缓蚀机理,结果表明,啤酒花单宁提取液是以阳极抑制为主的混合抑制型缓蚀剂,啤酒花单宁的吸附机理是单分子层吸附,符合Langmuir等温吸附方程。

啤酒花的HPLC指纹图谱建立及其抗氧化作用谱效关系研究

目的:建立啤酒花的高效液相色谱(HPLC)指纹图谱,并考察与其抗氧化作用的相关性。方法:色谱柱为Diamonsil C18,流动相为0.1%磷酸水溶液-乙腈(梯度洗脱),流速为1.0 m L/min,柱温为30℃,检测波长为358 nm,进样量为2μL。以黄腐酚峰为参照,绘制11批啤酒花药材样品的HPLC指纹图谱;采用《中药色谱指纹图谱相似度评价系统》(2012版)进行相似度评价,确定共有峰;以1,1-二苯基-2-三硝基苯肼(DPPH)自由基清除率、2,2′-连氨-(3-乙基苯并噻唑啉-6-磺酸)二氨盐(ABTS)自由基清除率为抗氧化作用的药效指标,采用SIMCA 14.1软件进行偏最小二乘回归分析以建立谱效关系,并进行体外抗氧化试验验证。结果:11批啤酒花药材样品共有19个共有峰,相似度均大于0.830。共指认出7个成分,分别为黄腐酚、类葎草酮、葎草酮、加葎草酮、类蛇麻酮、蛇麻酮和加蛇麻酮。11批啤酒花均具有清除DPPH和ABTS自由基的作用。谱效关系分析结果显示,啤酒花中黄腐酚、葎草酮、类蛇麻酮峰与其抗氧化能力呈正相关,且变量投影值均大于1。体外抗氧化验证结果显示,0.1 mg/mL黄腐酚与0.01 mg/mL维生素C对DPPH自由基的清除作用相当,但10.0 mg/mL黄腐酚对ABTS自由基清除作用小于0.1 mg/mL维生素C。结论:所建HPLC指纹图谱可用于评价啤酒花的质量;黄腐酚、葎草酮和类蛇麻酮可能是啤酒花具有抗氧化作用的物质基础。

酒花黄酮提取工艺和含量测定

建立酒花黄酮的提取方法和含量测定方法。采用NaNO2-Al(NO3)3-NaOH显色法,以芦丁为对照品,通过单因素试验和L9(34)正交设计确定酒花黄酮的提取方法,并测定和比较酒花、酒糟和啤酒中黄酮的含量。结果表明:酒花黄酮提取方法为样品加入50倍的甲醇,超声提取2次,每次1h,酒花黄酮含量为69.98mg/g,酒糟和啤酒中黄酮的含量较低。对照品芦丁在10.2～40.8μg/mL质量浓度范围内与吸光度呈良好线性关系,平均回收率99.33%,RSD=3.60%。该提取方法合理,含量测定方法简便、快速、准确,可用于酒花黄酮提取物制备及其质量控制。

啤酒花的地理分布与中国的野生啤酒花资源

啤酒花隶属于桑科葎草属,全世界共有该植物5变种,分布遍及北半球,间断分布于欧亚大陆和北美洲。作者通过对中国新疆地区啤酒花的实地调查,结合所搜集的啤酒花的文献资料,对啤酒花的起源,分化和地理分布进行讨论,并提出保护野生啤酒花资源的建议。

啤酒花中黄腐酚的生理活性作用的研究进展

黄腐酚为酒花中主要的异戊二烯基黄酮类物质。目前被发现仅存在于酒花中,其含量占酒花干重的0.1%～1%,它的结构赋予它多重生理活性。本文综述了近年来对酒花中黄腐酚的提取、分离纯化、结构鉴定、以及抗癌、抗病毒、预防动脉样硬化和糖尿病、雌性激素、抗氧化等生理活性及其作用机理的研究进展。

啤酒花多酚的提取工艺及抗氧化活性的研究

通过单因素和正交试验确定了酒花多酚的最佳提取工艺:浸提剂为70%丙酮,料液比1:25(g/ml),回流提取温度45℃,提取时间为1h,在此条件下多酚的提取量达到47.29mg/g干酒花。抗氧化实验结果显示酒花多酚对DPPH自由基的清除能力(IC506.72μg/ml)优于抗坏血酸(IC508.79μg/ml)和单宁酸(IC507.68μg/ml),弱于茶多酚(IC505.77μg/ml);酒花多酚的还原力(EC500.111mg/ml)与抗坏血酸(EC500.101mg/ml)接近,弱于单宁酸(EC500.079mg/ml)和茶多酚(EC500.072mg/ml);酒花多酚对小鼠肝匀浆脂质过氧化产生丙二醛(MDA)的抑制能力(IC500.179mg/ml)优于单宁酸(IC500.462mg/ml),弱于茶多酚(IC500.136mg/ml)。

啤酒花多酚类化合物提取工艺的优化研究

从提取溶剂及提取条件等方面对啤酒花多酚提取工艺进行了优化研究。用单因子试验对提取溶剂进行了筛选,结果表明丙酮和水组成的复合体系是理想的提取溶剂。用析因试验对提取条件进行了分析研究,结果表明丙酮浓度、提取温度、提取时间、料液比都对啤酒花多酚提取产生一定的影响,其中丙酮浓度和提取温度的影响最为显著。通过最陡爬坡试验和中心组合设计试验,优化得到最佳的多酚类化合物提取条件为:丙酮浓度为62%,提取温度为47℃,在此条件下啤酒花中多酚的最大提取量为47.40mg·g-1。

多效唑(MET)对啤酒花试管苗生长和移栽的影响

在培养基中加入 0 .1～ 0 .2 mg/L浓度的多效唑 ( MET) ,啤酒花试管苗植株矮壮 ,单株生根数量增加、移栽成活率提高 1 3%。 0 .5～ 2 .0 mg/L时 ,试管苗基部愈伤组织增多 ,枝叶失绿 ,生长受到抑制。

啤酒花的有效成分及活性研究

啤酒花是一种重要的传统中药,因其自身独特的药用价值而成为近来研究的热点.综述了国内外有关啤酒花的研究进展,涉及到化学成分,药理研究和临床应用,对啤酒花的医药研究与开发具有一定的参考价值.啤酒花含有树脂类、挥发油、黄酮类、鞣质、胆碱、粗纤维、氨基酸等多种化学成分.具有抗菌、抗肿瘤、抗氧化、雌性激素样、镇静等活性.在临床上可治疗结核、神经衰弱、麻风等多种疾病.

啤酒花茎段培养及快速繁殖技术研究

以啤酒花的幼嫩茎段作为外植体 ,研究出理想的一次性成苗培养基 :MS+ 6- BA 0 .0 1mg/ L+ IAA0 .1 mg/ L+琼脂 6.5g/ L+葡萄糖 2 %。试管苗月增殖率 4.2 ,生根率 1 0 0 % ,成苗率 90 %。采用试管苗微扦插的方式进行快速繁殖 ,经锻炼后直接移入经改造后的土壤中 ,移栽成活率达 93.8%。

啤酒花黄酮的研究进展

啤酒花黄酮是啤酒花中的一类小分子多酚类化合物,是代表该植物多种生物活性的一类重要活性成分。大多啤酒花黄酮在A环上有异戊烯基衍生的取代基,表现出抗病毒、抗真菌、抗疟原虫、抗肿瘤、抗NO生成、抗氧化、抑制骨吸收、雌激素样作用等多种生物活性,具有较好的开发利用前景。从化学结构、生物活性、体内外代谢等方面,归纳综述啤酒花黄酮的新近研究进展。

啤酒花中黄酮成分提取工艺的优化研究

目的:对啤酒花黄酮类化合物的提取工艺进行优化研究。方法:用单因素试验分别对提取溶剂乙醇含量、料液比、提取温度及提取时间进行研究,在此基础上通过正交试验确定上述4个因素的最佳组合。结果:优化后啤酒花中黄酮的最大提取量为78 mg.g-1。结论:啤酒花黄酮类化合物的适宜提取条件为乙醇含量45%、料液比1∶25、提取温度60℃、提取时间90 min。

啤酒花浸膏液态CO_2萃取及应用试验研究

开发生产国产液态ＣＯ２酒花浸膏具有重要意义。该文系统地进行了酒花浸膏的液态ＣＯ２萃取试验研究，通过啤酒发酵试验，研究并确认了在啤酒酿造中以自制酒花浸膏取代进口酒花浸膏的可行性结论。