Design,synthesis and anti-proliferative studies of a novel series of indirubin derivatives

A series of novel derivatives of indirubin were synthesized and evaluated for their anti-proliferative activity against human cancer cell lines of SGC7901,A549,HL-60,SK-BR-3 and HCT116.Most of the compounds displayed more potent activity than Sunitinib.In addition,the derivatives showed improved water solubility,which may be favorable to their pharmacokinetic performances.

Indirubin suppresses 4T1 murine breast cancer in vitro and in vivo by induction of ferroptosis

Objective Indirubin,isolated from Indigo Naturals,has been reported to have the inhibitory activity of MCF-7 human breast cancer cells in vitro.However,studies on its anti-breast cancer activity in vivo and the underlying mechanism are insufficient.We explored whether indirubin could trigger ferroptosis of breast cancer cells to exert anti-tumor activity.Methods Bioinformatical analysis was performed to detect the expression of prostaglandin-endoperoxide synthase 2(Ptgs2)in breast cancer tissues and Ptgs2-related prognosis for patients with breast cancer.The inhibitory effects of indirubin on 4T1 cells were assessed using MTT assay and LDH activity detection.The levels of 4-HNE,GPX4,PTGS2 and GSK-3βproteins were detected by Western blotting,and the mRNA of Ptgs2 was tested by qPCR.The contents of GSH and MDA were determined by commercial kits.Molecular docking was employed to study the interaction between indirubin and GSK-3β.A 4T1 murine breast cancer was adopted to evaluate the in vivo antitumor activity of indirubin.Results Indirubin promoted ferroptosis of 4T1 breast cancer cells with depleting of GSH,increased MDA and 4-HNE levels,as well as decreased GPX4 expression.Indirubin suppressed 4T1 breast tumor in vivo.The mechanism study showed indirubin up-regulated Ptgs2 expression by promoting phosphorylation(Ser 9)of GSK-3β.Conclusion Indirubin suppresses 4T1 murine breast cancer in vitro and in vivo by induction of ferroptosis.

Indirubin-3′-monoxime suppresses amyloid-beta-induced apoptosis by inhibiting tau hyperphosphorylation

Indirubin-3′-monoxime is an effective inhibitor of cyclin-dependent protein kinases, and may play an obligate role in neuronal apoptosis in Alzheimer＇s disease. Here, we found that indirubin-3′-monoxime improved the morphology and increased the survival rate of SHSY5 Y cells exposed to amyloid-beta 25–35（Aβ25–35）, and also suppressed apoptosis by reducing tau phosphorylation at Ser199 and Thr205. Furthermore, indirubin-3′-monoxime inhibited phosphorylation of glycogen synthase kinase-3β（GSK-3β）. Our results suggest that indirubin-3′-monoxime reduced Aβ25–35-induced apoptosis by suppressing tau hyperphosphorylation via a GSK-3β-mediated mechanism. Indirubin-3′-monoxime is a promising drug candidate for Alzheimer＇s disease.

Structural and Antileukemic Studies ofIndirubin Derivatives

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靛玉红(Indirubin)的含量测定

靛玉红是从中药青黛中提取分离得到的一种治疗慢粒白血病的有效成分。基于靛玉红分子中具有发色团的原理,藉此,作者以无水乙醇为溶媒,用72型分光光度计进行了比色法测定靛玉红含量的研究。作者进行了成色稳定性的考察;靛玉红标准曲线的制作;靛玉红回收率及加样回收率的测定;样品中微量靛蓝对靛玉红测定的影响;靛玉红片含量测定等工作。

STUDIES ON THE MECHANISM OF INDIRUBIN ACTION IN THE TREATMENT OF CHRONIC GRANULOCYTIC LEUKEMIA——V.BINDING BETWEEN INDIRUBIN AND DNA AND IDENTIFICATION OF THE TYPE OF BINDING

The binding between indirubin and calf thymus DNA in vitro has been verified by meansof the isotope labelling method, spectrophotometric method and thermal denaturation meas-urements. The λ_max 207 nm of indirubin shifted toward longer wave length with decrease ofabsorbance after the incubation of indirubin with DNA. The escalation of Tm value of DNAinduced by indirubin was about 2.4°C and it was reproducible. The binding force between themwas rather weak, as indirubin molecules were easily released during the precipitation withalcohol or the gel filtration. The binding was not affected by sodium chloride even at high con-centration but greatly decreased (to 20-30% of the control) in the presence of 8 M urea.These results showed that the binding between indirubin and DNA might be of hydrogen bondrather than ionic. The amount of bound ~3H-indirubin was directly proportional to the con-centration of indirubin. However, it increased abruptly when the concentration of indirubinreached 1.5×10^(-4) M. This suggested another binding force in the latter instance. By using spectrophotometric analysis and Scatchard plot it was found that calf thymusDNA bound 46 indirubin molecules/1000 nucleotides. The association constant (K) was5.7×10~6.

Molecular mechanism of indirubin-3＇-monoxime and Matrine in the reversal of paclitaxel resistance in NCI-H520/TAX25 cell line

Background Multidrug resistance （MDR） is a main reason for paclitaxel （TAX） treatment failure. Indirubin-3＇-monoxime （IRO） and Matrine are traditional Chinese medicines, which may reverse the resistance of tumor cells to some chemotherapy drugs, but the relationship between paclitaxel resistance and Matrine is still unclear. The aim of this study was to explore the potential molecular mechanism of IRO and Matrine in reversal of TAX resistance. Methods In this study, MTT assay was used to measure the non-cytotoxic dosage of IRO and Matrine on NCI-H520/TAX25 cells and determine the reversal extent of TAX resistance under non-toxic doses. In addition, RT-PCR and Western blotting were used to evaluate the mRNA expression and the protein level of survivin, Oct-4, and Sox-2 in NCI-H520fTAX25 ceils using semi-quantitative methods. Results There was no obvious inhibition on sensitive cell strains and drug-resistant strains, when the final concentration was at lest 4 IJmol/L for IRO and 100 IJmol/L for Matrine. So 4 tJmol/L of IRO and 100 pmol/L of Matrine were considered as the reversal dosage. When 4 IJmol/L of IRO or 100 pmol/L of Matrine were used together with TAX, the sensitivity to TAX increased evidently in NCI-H520/TAX2 cells; the reversal rate of IRO and Matrine was about 1.92 （43.56/22.6 nmol/L） and 1.74 （43.56/25.0 nmol/L）, respectively. The mRNA expression and the protein ievel of survivin, Oct-4, and Sox-2 in NCI-H520/TAX25 decreased significantly （P 〈0.05） after addition of IRO or Matrine in TAX treatment, compared to that of TAX treatment alone. Conclusion The decrease in both mRNA expression and protein level of survivin, Oct-4, and Sox-2 might be the molecular mechanism, by which IRO and Matrine mediate the reversal of TAX resistance.

FROM DANGGUI LONGHUI WAN TO BIOACTIVE INDIRUBIN ANALOGUES

Indirubin,indigo and isoindigo are the core representatives of a rather small category of bisindole alkaloids referred to as indigoids.These compounds are the coloured constituents of the natural dyes Indigo and the famous molluscan Tyrian purple,used throughout the centuries for textile dying.In contrast with Indigo dyes,the major constituents of molluscan purple dyes are

靛蓝提取物中靛蓝和靛玉红的分析方法比较

以靛膏为原料,采用盐酸酸化、葡萄糖还原和乙酸乙酯提取3种工艺制备靛蓝酸化物、靛蓝还原物和乙酸乙酯提取物。建立高效液相色谱(HPLC)法、紫外可见分光光度(UV)法和双波长紫外分光光度(dW-UV)法,分析3种靛蓝提取物中靛蓝和靛玉红的含量,并以Kolmogorov-Smirnov检验、Bland-Altman偏差图比较和Spearman检验确定3种样品各自最佳分析方法。结果表明:所建立的HPLC法、UV法和dW-UV法简单、准确、灵敏度高、稳定性好和重复性好。3种靛蓝提取物成分含量检测方法均遵从正态分布,两两测定值存在显著差异。UV法更适于分析靛蓝酸化物、靛蓝还原物中靛蓝含量;HPLC法更适于乙酸乙酯提取物中靛蓝、靛玉红含量分析。

基于Nrf2-HO-1/GPX4信号轴探讨中药靛玉红衍生物E804抑制肺癌A549细胞增殖和迁移的作用机制

目的 探讨中药靛玉红衍生物E804对非小细胞肺癌(NSCLC)系A549细胞增殖和迁移的影响,并阐明Nrf2-HO-1/GPX4信号轴可能的作用机制。方法 以肺癌A549细胞为细胞模型。采用MTT和细胞划痕实验观察0、10μmol/L E804和10μmol/L E804+不同特异性抑制剂(Nec-1、CQ、Z-VAD、DFO、Fer-1和Lip-1)组细胞的增殖和迁移能力;采用DCFH-DA荧光探针法检测0、2.5、5和10μmol/LE804组细胞内活性氧(ROS)含量,比色法检测二价铁离子(Fe^(2+))含量,分光光度法检测还原型谷胱甘肽(GSH)含量,微量法检测丙二醛(MDA)含量;Western blot法检测0、2.5、5和10μmol/L E804组细胞SLC7A11、Transferrin、GPX4、SLC40A1、Nrf2和HO-1蛋白表达水平。结果 与对照组(0μmol/LE804)比较,2.5、5和10μmol/L E804升高细胞内ROS、Fe^(2+)和MDA水平,降低细胞内GSH含量(P<0.01),同时降低SLC7A11、GPX4、SLC40A1、Nrf2和HO-1蛋白表达水平(P<0.01),升高Transferrin表达水平(P<0.05)。与单独使用10μmol/LE804组比较,细胞凋亡抑制剂(Z-VAD)组和细胞铁死亡抑制剂(DFO、Fer-1和Lip-1)组能够部分逆转E804对A549细胞的增殖和迁移抑制(P<0.01)。结论 E804可抑制A549细胞增殖和迁移,并诱发铁死亡,其机制可能与抑制Nrf2-HO-1/GPX4信号轴有关。

靛玉红通过下调Cyclin A2阻滞细胞周期抑制小鼠Lewis肺癌的体内外及网络药理学研究

目的研究中药成分靛玉红在体内外对小鼠Lewis肺癌(LLC)的抑制效果及对细胞周期的调节作用。方法通过细胞毒性实验探究靛玉红在体外对小鼠LLC细胞的抑制作用。构建肺癌原位小鼠模型,随机分为模型组(磷酸盐缓冲液灌胃,每天1次)和靛玉红低、中、高剂量组(25 mg/kg、50 mg/kg、100 mg/kg灌胃,每天1次)、顺铂组(2 mg/kg腹腔注射,每3天1次),连续3周,记录生存期和体质量。通过活体成像法记录小鼠肺癌进展,取肺肿瘤组织,称重并计算抑瘤率。通过网络药理学预测靛玉红治疗肺癌的核心靶点和通路。Western blot法分别验证靛玉红在体外对LLC细胞及在体内对小鼠肺癌组织中细胞周期蛋白A2(Cyclin A2)表达的影响;免疫组织化学染色(IHC)法和实时荧光定量逆转录聚合酶链式反应(RT-qPCR)法分别检测靛玉红对小鼠肺癌组织中Cyclin A2蛋白及其编码基因CCNA2表达的影响。流式细胞术和IHC法分别检测靛玉红对小鼠肺癌肿瘤细胞的细胞周期和肺癌肿瘤增殖抗原Ki-67表达的影响。结果靛玉红在体外对小鼠LLC细胞的抑制作用呈剂量和时间依赖性,24 h、48 h、72 h的半抑制浓度(IC_(50))分别为188.7μmol/L、109.0μmol/L、58.3μmol/L。与模型组比较,靛玉红中剂量组小鼠肺部荧光表达降低(P<0.05),生存率提高(中位生存期延长7 d),肿瘤抑制率较高(37.76%),且对小鼠体质量没有明显影响(P>0.05)。网络药理学分析表明,靛玉红抑制肺癌可能通过调控细胞周期及Cyclin A2实现。进一步研究证明,靛玉红通过抑制Cyclin A2,导致细胞周期S期阻滞,抑制肿瘤细胞增殖。结论靛玉红体外抑制小鼠LLC细胞,体内通过下调肺癌肿瘤细胞Cyclin A2导致细胞周期阻滞,抑制肿瘤进展,延长肺癌小鼠生存期。

基于信号通路探讨青黛治疗溃疡性结肠炎的研究进展

溃疡性结肠炎(ulcerative colitis,UC)是一种慢性非特异性炎症,中医药对UC的疗效确切。中药青黛发挥多靶点、复发率低、毒副作用较小的独特优势,对UC有较快缓解作用。青黛治疗UC微观分子机制可能涉及芳香烃受体/白介素-22(aryl hydrocarbon receptor/interleukin-22,AhR/IL-22)、核因子—红细胞2型相关因子/血红素氧合酶-1(nuclear factor erythroid 2-related factor 2/heme oxygenase-1,Nrf2/HO-1)、Janus激酶/信号转导和转录激活因子3(janus kinase/signal transducer and activator of transcription 3,JAK/STAT3)、转化生长因子β/Smad(transforming growth factorβ,TGF-β/Smad)、磷脂酰肌醇-3-激酶(phosphoinositide 3-kinase,PI3K)/蛋白激酶B(protein kinase B,Akt)、有丝分裂原活化蛋白激酶(mitogen-activated protein kinase,MAPK)信号通路、核因子-κB(nuclearfactor kappa-B,NF-κB)7条信号通路。大量动物实验、细胞实验证明,青黛及活性成分可通过直接作用于AhR然后激活AhR/IL-22信号通路,调节免疫反应,加强肠黏膜屏障功能;通过Nrf2/HO-1信号通路发挥抗氧化应激保护肠道屏障;通过JAK/STAT3信号通路调节辅助性T淋巴细胞17/调节性T淋巴细胞免疫平衡;通过NF-κB、MAPK信号通路发挥抗炎、抗细胞焦亡、保护紧密连接屏障作用;通过PI3K/Akt信号通路调节凋亡蛋白表达,预防UC相关癌症进展;通过TGF-β/Smad信号通路调节炎症因子,预防肠道纤维化等。现代分子生物学研究证实青黛及主要成分可通过调节相关信号通路相关分子的表达,降低肠道细胞的异常凋亡、分化及相关炎性因子的转录与释放,改善肠道稳态,加速溃疡愈合。本综述系统阐述青黛通过各信号通路调节机体免疫反应治疗UC,充分挖掘青黛活性成分及方剂的作用机制,为中医药发展提供理论基础。

板青颗粒特征图谱及其质量相关性研究

本研究旨在开发一种用于检测板青颗粒中靛玉红含量的方法,并进行指纹图谱分析。采用高效液相色谱技术,色谱柱选用Eclipse Plus C_(18)柱(4.6 mm×250.0 mm,5μm),检测波长289 nm,以甲醇-水(77∶23)为流动相,等度洗脱,流速为0.8 mL/min,柱温30℃,进样量10μL。结果显示,在对靛玉红定性分析中线性关系良好(R^(2)=1.0000),平均回收率为98.07%,12批次样品中检测出共有峰7个,相似度为0.791~1.000。该方法操作简单、快捷,结果准确,可用于板青颗粒中靛玉红含量的测定及板青颗粒质量评价。

靛玉红可能通过靶向MAPK14参与银屑病的发病

目的探讨靛玉红在银屑病中的作用靶点,初步阐明靛玉红在银屑病中可能通过MAPK14对银屑病产生的影响。方法从高通量基因表达(GEO)数据库下载GSE30999和GSE78097银屑病数据集,分别作为训练集和验证集。筛选出差异表达基因,然后分析其生物学功能和通路。与靛玉红靶点基因取交集获取差异表达的靛玉红靶点基因,分析基因的相关性和验证基因差异表达情况。采用LASSO回归模型和Cox回归模型筛选靛玉红的最佳靶点基因,与靛玉红进行分子对接分析两者之间的结构关系。结果在GSE30999数据集中,共发现8个靛玉红靶点基因,与对照组相比,均有差异表达。其中7个基因均具有较高的诊断价值(AUC均>0.8),1个基因具有较低诊断价值(AUC>0.6)。GO和KEGG富集分析显示靛玉红的8个靶点基因主要与细胞衰老、化学致癌-受体激活、脂质与动脉粥样硬化、急性髓系白血病和AGE-RAGE信号通路在糖尿病并发症中的作用有关。通过LASSO回归模型和Cox回归模型筛选了靛玉红的最佳靶点基因——MAPK14基因。分子对接显示靛玉红与MAPK14紧密结合。结论靛玉红可能通过MAPK14参与银屑病发病机制的调控和治疗。

酶法辅助提取南板蓝叶中靛玉红的工艺研究

[目的]研究酶法提取关键参数对南板蓝叶中靛玉红提取工艺的影响。[方法]采用HPLC测定靛玉红的含量,并考察酶用量、酶解pH值和酶解时间对提取率的影响,并优选出了最佳工艺条件。[结果]南板蓝叶中靛玉红酶法辅助提取的最佳工艺条件为:酶用量25 U/g,酶解pH值4.8,酶解时间6 h;在此条件下,靛玉红的Z值为7.02%。[结论]酶法辅助提取法适用于南板蓝叶中靛玉红的提取。

运用近红外光谱技术快速测定大青叶中靛玉红含量

目的运用近红外光谱技术快速测定大青叶中靛玉红含量,建立靛玉红的近红外定量分析模型,并通过模型分析评价大青叶的品质。方法采用传统的高效液相色谱法对74批大青叶中靛玉红含量进行测定及方法学验证,运用偏最小二乘法建立靛玉红含量与近红外光谱之间的定量校正分析模型,并对验证集样品进行含量预测,将预测值与实际测定值进行统计分析。结果靛玉红浓度在1.04~3.13μg·ml^(-1)范围内线性良好,回归方程为Y=11566X+911.7,r=0.9990;精密度、重复性、12 h内稳定性的RSD分别为0.31%、0.86%、1.11%;加样平均回收率为99.22%。建立的定量分析模型准确性好,内部交叉验证均方差、内部交叉验证决定系数分别为0.226、0.983。通过对24份校正集样品进行外部验证,近红外预测值与高效液相测定值的预测回收率为93.66%。对两组数据进行方差显著性分析,其显著性指标值分别为0.540和0.428,表明两种试验方法的数据差异无统计学意义,该模型的精度和再现性均符合规定。结论近红外光谱技术对大青叶中靛玉红含量测定结果较好,建立的定量分析模型可以无损、快速、准确地对大青叶进行质量评价,提高生产效率。

复方黄黛片有效成分纳米粒的制备及其肝癌治疗研究

目的探讨复方黄黛片有效成分硫化砷、靛玉红和丹参酮联合装载纳米粒的制备及肝癌HepG2和Huh-7细胞的治疗作用。方法应用单乳溶媒挥发法,制备聚乳酸-聚羟基乙酸共聚物联合装载硫化砷、靛玉红和丹参酮纳米粒。氢化物发生原子吸收分光光度法和高效液相色谱法分析纳米粒中药物的载药率、包封率和模拟体外释药,利用扫描电镜观察纳米粒的形态,采用粒度分析仪检测纳米粒粒径。荧光显微镜观察HepG2和Huh-7细胞吞噬摄取纳米粒,采用MTT测定法检验细胞活力,细胞存活分析检测细胞克隆形成能力。结果联合载药纳米粒呈球形,粒径为(115.09±36.71)nm,多分散指数0.131。硫化砷、靛玉红和丹参酮的载药率和包封率分别为(5.17±1.26)%、(1.03±0.45)%、(1.72±0.67)%和(16.15±4.7)%、(76.74±6.8)%、(83.09±9.4)%。硫化砷、靛玉红和丹参酮模拟体外释药曲线早期呈爆发释放,随后为缓慢持续释放。荧光显微镜结果可见肝癌细胞对纳米粒的吞噬摄取,MTT检测显示药物单体和联合载药纳米粒作用后细胞活力较对照降低,联合载药纳米较药物单体粒作用显著,细胞存活分析结果也进一步证实上述结果。结论复方黄黛片有效成分硫化砷、靛玉红和丹参酮联合装载纳米粒显示出明确的肝癌治疗效果,这为中药的临床给药提供了新的剂型。

HPLC测定板蓝根提取物中靛蓝和靛玉红的含量

目的 采用HPLC测定板蓝根提取物中靛蓝和靛玉红含量。方法 将板蓝根醇提液挥去乙醇 ,经氯仿萃取 ,然后用HPLC测定。色谱柱为DikmaDiamonsilTMC18(5 μm ,2 0 0mm× 4 6mm) ,流动相为甲醇 - 0 1%醋酸铵 -醋酸 (70∶30∶1) ,流速为1 0ml·min-1,检测波长 2 80nm。结果 靛蓝线性范围在 0 0 15 2～ 0 30 4 0 μg(r =0 9997) ,平均加样回收率为 97 3% ,RSD =1 87% (n =5 ) ;靛玉红线性范围在 0 0 16 5 6～ 0 3312 μg ,平均加样回收率为 96 6 % ,RSD =2 .32 % (n =5 )。结论 所用方法简便快捷 ,适合板蓝根药材以及含靛蓝、靛玉红产品的质量控制。

逆境胁迫对菘蓝幼苗靛玉红含量的影响

培养30d的菘蓝无菌幼苗经250mmol／L NaCl、自然干旱、20mmol／L ABA、4℃低温等不同方式逆境处理，不同时间内取样，用高效液相色谱法对其中靛玉红的含量进行测定。结果表明：盐、干旱、ABA处理12h内能提高菘蓝幼苗中靛玉红含量59.05％～161．67％，低温胁迫处理24h也能提高靛玉红含量141．4％，说明适当逆境胁迫处理能有效提高菘蓝幼苗体内靛玉红的累积量，其中250mmol／L NaCl胁迫处理效果最为显著。

小檗碱、吴茱萸碱和靛玉红对人胃癌细胞的作用比较

目的:探讨加味左金丸三种组成中药的主要单体成分小檗碱、吴茱萸碱和靛玉红对人胃癌细胞生长抑制、诱导凋亡和细胞周期的影响. 方法:人胃癌细胞株为低分化黏液腺癌MGC803细胞; 小檗碱、吴茱萸碱和靛玉红购自中国药品与生物制品检定所.苔盼蓝染色细胞计数法测定细胞存活率和凋亡率,流式细胞技术进行细胞周期、凋亡百分比分析,甲基绿-派诺宁联合染色法观测凋亡形态,琼脂糖凝胶电泳分析DNA损伤情况. 结果:96 h内小檗碱、吴茱萸碱各组细胞存活率不断下降,其中48 h存活率对照组为100.0±7.9%,小檗碱4 mg/L和8 mg/L组分别为72.9±6.2%(t=4.67, P<0.01)和17.4±4.8%(t=15.48,P<0.001),吴茱萸碱1 mg/L和5 mg/L组分别为37.8±5.7%(t=11.06, P<0.001)和10.7±11.1%(t=11.35,P<0.001);各组均与对照组比较(n=3);对生长的抑制作用呈时间、药物浓度依赖性.甲基绿-派诺宁原位染色,细胞表现出凋亡特征.小檗碱与吴茱萸碱组脱落的悬浮死细胞中有较高比例胞膜完整、抗拒苔盼蓝和酚红染色的凋亡细胞, 其中48 h凋亡率对照组为0.3±0.0%,小檗碱8 mg/L 组为65.2±9.5%(t=11.83,P<0.001);吴茱萸碱1 mg/L组为58.9±11.4%(t=8.90,P<0.001),而阿霉素组脱落死细胞不能抗拒苔盼蓝和酚红染色.流式细胞仪检测表明小檗碱与吴茱萸碱组均出现亚二倍体凋亡峰;细胞周期分别阻滞于G0—G1、G2期;凋亡百分比与对照组11.8±2.5比较,小檗碱4 mg/L组48 h 为18.9±2.7(t=3.34,P<0.05),72 h为23.9±3.3(t=5.06,P<0.01),吴茱萸碱1 mg/L组72 h 为16.6±1.6(t=2.80,P<0.05).琼脂糖凝胶电泳表明,小檗碱组DNA裂成大片段,吴茱萸碱组和阿霉素组DNA断裂呈涂抹状.靛玉红各组对细胞生长、凋亡无影响,DNA无损伤. 结论:小檗碱与吴茱萸碱均能诱导人胃癌细胞凋亡,且作用较阿霉素温和;靛玉红对胃癌细胞的体外作用不明显.