Combination immunotherapy with Survivin and luteinizing hormone-releasing hormone fusion protein in murine breast cancer model

AIM To investigate the therapeutic potential of two recombinant proteins, Survivin and luteinizing hormone-releasing hormone (LHRH) fusion protein [LHRH(6 leu)-LTB] for immunotherapy of breast cancer.METHODS Murine 4 T-1 breast cancer model was used to evaluate the efficacy of recombinant proteins in vivo. Twenty four Balb/c mice were divided into 4 groups of 6 mice each. Recombinant Survivin and LHRH fusion protein, alone or in combination, were administered along with immunomodulator Mycobacterium indicus pranii (MIP) in Balb/c mice. Unimmunized or control group mice were administered with phosphate buffer saline. Each group was then challenged with syngeneic 4 T-1 cells to induce the growth of breast tumor. Tumor growth was monitored to evaluate the efficacy of immune-response in preventing the growth of cancer cells.RESULTS Preventive immunization with 20 μg recombinant Survivin and MIP was effective in suppressing growth of 4 T-1 mouse model of breast cancer (P = 0.04) but 50 μg dose was ineffective in suppressing tumor growth. However, combination of Survivin and LHRH fusion protein was more effective in suppressing tumor growth (P = 0.02) as well as metastasis in vivo in comparison to LHRH fusion protein as vaccine antigen alone.CONCLUSION Recombinant Survivin and MIP suppress tumor growth significantly. Combining LHRH fusion protein with Survivin and MIP enhances tumor suppressive effects marginally which provides evidence for recombinant Survivin and LHRH fusion protein as candidates for translating the combination cancer immunotherapy approaches.

Long-term effectiveness of luteinizing hormone-releasing hormone agonist or antiandrogen monotherapy in elderly men with localizect prostate cancer （T1-2） ： a retrospective study

Aim： To evaluate the long-term effectiveness, side effects and compliance rates of two types of drugs （luteinizing hormone-releasing hormone [LHRH] agonist and antiandrogen） that were used individually to treat patients with localized prostate cancer （T1-2） at our institution. Methods： Ninety-seven patients who were diagnosed in the period from April 1997 to January 2000 as having clinically localized prostate cancer （T1-2） received either LHRH agonist （leuprolide acetate 7.5 mg/month） monotherapy （group 1, n = 62） or antiandrogen monotherapy （group 2, n = 35; 18 received bicalutamide 50 mg q.d., 13 received nilutamide 150 mg t.i.d, and 4 received flutamide 250 mg t.i.d.）. The mean age in both groups was 76 years. Results： The mean follow-up time was （50.8 ±8.5） months in group 1 and （43.1 ± 2.2） months in group 2. Prostate-specific antigen （PSA） levels rose in only 1 of the 62 patients （1.6%） in group 1, and in 20 of the 35 patients （57.1%） in group 2. In group 2, 10 of the 20 patients （50 %） with increasing PSA levels were treated with LHRH salvage therapy, and eight （80%） responded. Hot flashes （54.8%） and lethargy （41.9%） were the most common side effects in group 1. In contrast, nipple-tenderness （40%） and light-dark adaptation （17.1%） were more often seen in group 2. Only 1 of the 62 patients （1.6%） in group 1 switched to another medication because of adverse side effects; whereas 8 of the 35 patients （22.9%） in group 2 did so. Conclusion： Unlike antiandrogen monotherapy, LHRH agonist monotherapy provided long-term durable control of localized prostate cancer （T1-2）. It can also be an effective treatment option for patients whose disease failed to respond to antiandrogen monotherapy. The limitations of our study are the lack of health outcomes analysis and a small sample size.

Effect of Luteinizing Hormone-Releasing Hormone Analogue on the Sexual Behavior of Sacalia quadriocellata

Luteinizing hormone-releasing hormone(LHRH) is known to influence sexual behavior in many vertebrate taxa, but there have been no systematic studies on the role of LHRH in sexual behavior of turtles. We tested the hypotheses that exogenous LHRH analogues would induce sexual behavior of male Four-eyed turtle, Sacalia quadriocellata. We examined this by challenging males with intramuscular injections of mammalian luteinizing hormone-releasing hormone analogue(LHRH-A), human chorionic gonadotropin(HCG), or a combination of the two, and subsequently exposing them to sexually receptive females for behavioral observation. Our data show that the injection of only HCG could not, while that of only LHRH-A could, facilitate sexual behavior along with testicular recrudescence and spermatogenesis in S. quadriocellata. The injection of both LHRH-A and HCG would induce more drastic sexual behavior of the animals than that of LHRH-A alone, indicating HCG enhances the effects of LHRH-A induced sexual behavior. However, different pharmacological dosages of LHRH-A(0.5 μg, 1 μg, 2 μg per 100 g bodyweight) did not correspond to different activity levels. Though the mechanism of LHRH effect was not determined, this study may support that the sexual behavior of S. quadriocellata which occurs at the beginning of the injection despite regression of the gonads. This is the first report on the exogenous LHRH-A induced sexual behavior for this species.

Morphological changes of gonadotropin-releasing hormone neurons in the rat preoptic area across puberty

Gonadotropin-releasing hormone （GnRH） neurons in the preoptic area may undergo morphological changes during the pubertal period when their activities are upregulated. To clarify the regulatory mechanism of puberty onset, this study aimed to investigate the morphological changes of GnRH neurons in the preoptic area of GnRH-enhanced green fluorescent protein transgenic rats. Under confocal laser microscopy, pubertal GnRH neurons exhibited an inverted Y distribution pattern. Prepubertal GnRH neurons were generally unipolar and bipolar, and were distinguished as smooth type cells with few small processes or irregular type cells with many spine-like processes in the proximal dendrites. The number of GnRH neurons in the preoptic area and spine-like processes were increased during the course of reproductive maturation. There was no significant difference between male and female rats. Immunofluorescence staining revealed synaptophysin punctae close to the distal end of GnRH neurons, indicating that some presynaptic terminals may form a synaptic linkage with these neurons.

Kisspeptin regulates gonadotropin-releasing hormone secretion in gonadotropin-releasing hormone/enhanced green fluorescent protein transgenic rats

Kisspeptin is essential for activation of the hypothalamo-pituitary-gonadal axis. In this study, we established gonadotropin-releasing hormone/enhanced green fluorescent protein transgenic rats. Rats were injected with 1, 10, or 100 pM kisspeptin-10, a peptide derived from full-length kisspeptin, into the arcuate nucleus and medial preoptic area, and with the kJsspeptJn antagonist peptJde 234 into the lateral cerebral ventricle. The results of immunohistochemical staining revealed that pulsatile luteinizing hormone secretion was suppressed after injection of antagonist peptide 234 into the lateral cerebral ventricle, and a significant increase in luteinizing hormone level was observed after kisspeptin-10 injection into the arcuate nucleus and medial preoptic area. The results of an enzyme-linked immunosorbent assay showed that luteinizing hormone levels during the first hour of kisspeptin-10 infusion into the arcuate nucleus were significantly greater in the 100 pM kisspeptin-10 group than in the 10 pM kisspeptin-10 group. These findings indicate that kisspeptin directly promotes gonadotropin-releasing hormone secretion and luteinizing hormone release in gonadotropin-releasing hormone/enhanced green fluorescent protein transgenic rats. The arcuate nucleus is a key component of the kisspeptin-G protein-coupled receptor 54 signaling pathway underlying regulating luteinizing hormone pulse secretion.

Preclinical therapy of benign prostatic hyperplasia with neuropeptide hormone antagonists

Benign prostatic hyperplasia(BPH)is a pathologic condition of the prostate described as a substantial increase in its number of epithelial and stromal cells.BPH may significantly reduce the quality of life due to the initiation of bladder outlet obstruction and lower urinary tract syndromes.Current medical therapies mostly consist of inhibitors of 5α-reductase orα1-adrenergic blockers;their efficacy is often insufficient.Antagonistic analogs of neuropeptide hormones are novel candidates for the management of BPH.At first,antagonists of luteinizing hormone-releasing hormone(LHRH)have been introduced to the therapy aimed to reduce serum testosterone levels.However,they have also been found to produce an inhibitory activity on local LHRH receptors in the prostate as well as impotence and other related side effects.Since then,several preclinical and clinical studies reported the favorable effects of LHRH antagonists in BPH.In contrast,antagonists of growth hormone-releasing hormone(GHRH)and gastrin-releasing peptide(GRP)have been tested only in preclinical settings and produce significant reduction in prostate size in experimental models of BPH.They act at least in part,by blocking the action of respective ligands produced locally on prostates through their respective receptors in the prostate,and by inhibition of autocrine insulin-like growth factors-Ⅰ/Ⅱand epidermal growth factor production.GHRH and LHRH antagonists were also tested in combination resulting in a cumulative effect that was greater than that of each alone.This article will review the numerous studies that demonstrate the beneficial effects of antagonistic analogs of LHRH,GHRH and GRP in BPH,as well as suggesting a potential role for somatostatin analogs in experimental therapies.

LHRH-A缓释剂促进雄性赤点石斑鱼性类固醇激素分泌和精巢发育与排精的研究

研究了促黄体生成素释放激素类似物(LHRHA)不同处理方式对雄性赤点石斑鱼性类固醇激素分泌和精子生成及精子排放的影响。对照组在0、7d二次注射生理盐水(50μg·kg-1BW),注射组在0、7d二次注射LHRHA(50μg·kg-1BW),埋植组在0d埋植LHRHA缓释剂(100μg·kg-1BW)。结果表明,通过埋植LHRHA缓释剂,血清睾酮(T)和11-酮基睾酮(11-KT)水平快速增加,显示血清睾酮和11-酮基睾酮水平与赤点石斑鱼精子生成和精子排放有密切关系。组织学观察表明,在21d,对照组和注射组鱼精巢充满了精子细胞、精母细胞和精原细胞,而在同一时间,LHRHA埋植组鱼精巢含有大量精子,表明精子排放仍在进行。在40d期间采集精液总量为对照组<注射组<埋植组,差异显著。当注射组在处理14d后精液量逐渐回落到对照组水平时,埋植组仍然维持较高精液量水平。各组采集的精子的活力与采集的精液量呈正相关,而精子密度没有显著差异。数据显示,LHRHA缓释剂能显著增加赤点石斑鱼的精液量及延长精子排放时间而不改变精子的质量。

半胱胺盐酸盐和LHRH-A对黄鳍鲷IGF-Ⅰ基因表达和生长的影响

本文以黄鳍鲷 (Sparuslatus)为研究对象 ,利用GeneRaceTM 技术 ,从其肝组织中克隆出类胰岛素生长因子 (IGF Ⅰ )cDNA ,并应用半定量RT PCR方法研究了半胱胺盐酸盐 (Cysteaminehydrochloride)和LHRH A对其肝组织IGF Ⅰ基因表达的影响。黄鳍鲷IGF ⅠcDNA全长为 84 0bp ,编码 185aa多肽 ;序列分析表明 ,黄鳍鲷IGF Ⅰ基因编码的氨基酸序列与金鱼的同源性为 75 8% ,与牙鲆的同源性为 86 5 % ,与同属鲷科的黑鲷同源性高达 10 0 % ,证明鱼类类胰岛素生长因子是非常保守的 ,E区域分析结果表明黄鳍鲷IGF Ⅰ属Ea 4型。在饲料中投喂CSH、LHRH A等添加剂 ,实验组黄鳍鲷鱼种的相对生长率、垂体GH含量、肝脏IGF ⅠmRNA水平均显著高于对照组。以上结果提示 :CSH、LHRH A能促进黄鳍鲷生长激素的合成和IGF Ⅰ基因的表达 。

LHRH-PE40与Hela细胞表面LHRH受体结合的特异性及其细胞毒性

目的:研究重组免疫毒素LHRH -PE40与Hela细胞表面LHRH受体结合的特异性,并观察由此产生的细胞毒性作用。方法:ELISA方法检测LHRH- PE40与Hela细胞表面LHRH受体结合的高度特异性、饱合性及其与时间的关系;LHRH- PE40由LHRH受体介导对Hela细胞产生细胞毒作用进行光、电镜观察。结果:LHRH -PE40与Hela细胞表面受体的结合与正常鸡胚成纤维细胞的结合相比有显著意义(P<0. 01);LHRH- PE40与LHRH竞争LHRHR的OD值和TSH相比有显著意义(P<0. 01);光镜观察,LHRH- PE40对Hela细胞作用明显而对正常鸡胚成纤维细胞几乎没有作用;电镜观察,LHRH -PE40使Hela细胞表面出现凋亡征象。结论:与其他正常组织的细胞相比, Hela细胞膜表面LHRH受体分布呈过表达状; LHRH -PE40与细胞表面LHRH受体的结合具有高度特异性、饱和性; LHRH -PE40对细胞的作用由LHRHR介导,并且只对LHRHR阳性细胞产生毒性作用。

LHRH-A缓释剂对雌性赤点石斑鱼卵巢发育、性类固醇激素分泌及脑垂体GTH细胞超微结构的影响

取75尾网箱养殖的2～3龄雌性赤点石斑鱼,分为3组(高、低剂量组和对照组),各25尾。高剂量组埋植促黄体生成素释放激素类似物(LHRHA)缓释剂,剂量为300μg/kg体重,低剂量组为100μg/kg体重,对照组埋植不含LHRHA的药丸。分别在实验开始和埋植药丸后0、10、20、30、40天抽血,用放射免疫测定血清类固醇激素(E2、T);解剖鱼体测定相关指标,计算性腺成熟系数;取性腺和肝脏组织常规组织学切片并透射电镜观察。埋植后第10—30天,两种剂量处理组的排卵率均高于对照组,高剂量组显著高于低剂量组。在第10天性腺成熟系数高剂量组为1.055%,卵母细胞已有部分迅速发育到Ⅳ期末(核偏位);低剂量组相对缓慢。第20天性腺成熟系数高剂量组达1.858%,低剂量组为0.987%;处理组卵母细胞基本发育成熟。埋植后第10天,两处理组血清E2和T水平显著升高;第20天显著下降;此后E2保持在较低的水平,T显著低于对照组水平。超微结构的观察证实脑垂体GTH细胞在LHRHA缓释剂诱导性腺发育成熟和排卵过程中处于活跃的合成与分泌状态。LHRHA缓释剂能有效诱导赤点石斑鱼卵巢发育成熟和排卵,而性类固醇激素(E2、T)只与卵黄生成有关,与排卵无关。

DAB389-Linker-LHRH重组毒素的构建及生物活性的初步测定

采用基因工程方法,将白喉毒素的毒性部分(DAB389)通过柔性连接肽(Linker)与促黄体激素释放素(LHRH)基因连接起来,克隆到高效表达载体pET28a(+)中,并在大肠杆菌中表达该融合蛋白(DAB389-Linker-LHRH).通过三步层析纯化目的蛋白,获得了纯度达95%的重组毒素DAB389-Linker-LHRH.用MTT法检测其对过度表达LHRH受体的人宫颈癌HeLa细胞的毒性作用,探讨其对HeLa细胞的特异杀伤情况.实验结果显示DAB389-Linker-LHRH对HeLa细胞具有很强的生长抑制作用,其IC50为12.93μg/mL.表明该免疫重组毒素在体外对人宫颈癌HeLa细胞具有明显的杀伤作用,为进一步研制对宫颈癌有特异治疗作用的靶向抗癌药物奠定了基础.

LHRH刺激雄性大鼠垂体LH分泌高峰时细胞形态变化的图象分析

应用ABC亲和组织化学顺序、MIS－I计算机图象处理系统测定外源性LHRH刺激雄性大鼠LH分泌高峰前后LH细胞面积、细胞内液泡面积和细胞形状等形态参数的变化。结果表明：雄性大鼠LH基础分泌时，LH细胞处于贮存状态：大细胞（＞340μm2）占LH阳性细胞56．7％，小细胞（＜190μm2）占2．2％，40％细胞内含有大量液泡，细胞形状大多偏向圆形。注射LHRH30min后，血中LH浓度显著升高，LH细胞平均面积明显减小；60min时，血中LH释放达到高峰，相应的形态学特征是大细胞降低至4％，小细胞增加到66％。随着细胞内液泡的大量消失，52．6％的细胞偏向不规则形状。LH分泌高峰后，血液LH浓度逐渐恢复到基础分泌水平，但随着细胞内LH贮存的增加，细胞和细胞内液泡平均面积逐渐增加，大多数细胞又偏向圆形。结果提示，合大量液泡的偏圆形大细胞同LH大量贮存有关。而液泡的消失以及大量小细胞和不规则形状细胞的出现同LH大量释放有密切联系。由此作者认为：LH细胞内液泡的动态变化以及由此产生的细胞大小、细胞形状和细胞结构的变化可以作为促性腺激素分泌的重要形态学观察指标。

LHRH及P物质对大鼠脊神经节细胞膜GABA_A受体介导反应的抑制作用

实验在幼年大鼠脊神经节（ＳＧ）标本进行细胞内记录。结果表明，单独滴加０．０１～１．００ｍｍｏｌ／Ｌγ－氨基丁酸（ＧＡＢＡ）在大多数受检细胞（１０６／１２７）引起荷包牡丹碱敏感的去极化，而胞体膜对０．０１～０．１０ｍｍｏｌ／Ｌ促性腺素释放激素（ＬＨＲＨ）或０．００１～０．０１ｍｍｏｌ／ＬＰ物质（ＳＰ）仅有轻微的去极化或无反应。若将此两种肽类物质在ＧＡＢＡ作用之前分别加至ＳＧ细胞，这时ＧＡＢＡ所引起的反应便大为减弱。结果提示，肽类物质ＬＨＲＨ及ＳＰ对ＧＡＢＡ_Ａ受体介导的初级传入终末突触前抑制具有调制作用。

LHRH-PE40对宫颈癌细胞株细胞周期及Ki-67、Bcl-2的影响

目的观察LHRH-PE40对宫颈癌Hela细胞系凋亡及增殖的影响,为其临床应用提供理论依据。方法采用人宫颈癌Hela细胞株进行培养,在培养液中分别加入不同浓度的LHRH-PE40,作用48h后,观察Hela细胞形态的变化,并通过结晶紫染色法检测宫颈癌Hela细胞株对LHRH-PE40的感受性;用流式细胞仪及免疫组化法检测LHRH-PE40对Hela细胞周期、Ki-67及Bcl-2的影响。结果LHRH-PE40对Hela细胞活性的抑制作用呈剂量依赖性,通过量效曲线可以看出,LHRH-PE40的最小有效剂量为0·625μg/ml;半数致死剂量为0·969μg/ml。在1·0μg/ml浓度下,癌细胞中的Ki-67阳性细胞(用药前80%,用药后42%)及Bcl-2阳性细胞(用药前66%,用药后43%)比率均下降,凋亡细胞比率增加(由0增加到3·7%)。在1·0μg/ml浓度下,细胞的G0/G1期细胞比率增加15·21%;S期细胞变化不大,而G2/M期减少38·28%。结论LHRH-PE40可以有效地抑制宫颈癌细胞的增殖,诱发肿瘤细胞凋亡,是一种很有应用前景的抗肿瘤药物。

中枢性性早熟及外周性性早熟女童的LH、LHRH水平变化及临床意义

目的研究中枢性性早熟及外周性性早熟女童的黄体生成素(LH)、黄体生成素释放激素(LHRH)水平变化及临床意义。方法回顾性分析2018年1月至2021年12月在惠州市第一人民医院儿科诊治的54例性早熟女童的临床资料,按照早熟性质分为中枢性组(中枢性性早熟,35例)与外周性组(外周性性早熟,19例)。采用化学发光免疫法检测所有女童的LH、睾酮(T)、雌二醇(E2)、卵泡刺激素(FSH)水平及LHRH激发试验中的LH、FSH水平,计算并比较两组女童的骨龄指数、子宫容积和卵巢容积。结果中枢性组女童的LH、FSH水平分别为(4.35±1.54)IU/L、(7.28±2.11)IU/L,明显高于外周性组的(2.34±1.03)IU/L、(4.60±1.32)IU/L,T水平为(12.41±19.22)μg/L,明显低于外周性组的(84.46±123.24)μg/L,差异均有统计学意义(P<0.05);中枢性组女童的E2水平为(16.73±23.60)ng/L,与外周性组的(32.24±42.24)ng/L比较差异无统计学意义(P>0.05);LHRH激发试验分别30 min、60 min、90 min,中枢性组女童的LH水平分别为(19.53±2.66)IU/L、(16.15±2.12)IU/L、(12.45±1.86)IU/L,均明显高于外周性组的(5.65±1.78)IU/L、(5.38±1.40)IU/L、(4.26±1.17)IU/L,差异均有统计学意义(P<0.05);LHRH激发试验分别30 min、60 min、90 min,中枢性组女童的FSH水平分别为(15.24±5.28)IU/L、(15.90±5.06)IU/L、(15.99±5.40)IU/L,均明显高于外周性组的(10.96±3.27)IU/L、(11.23±3.74)IU/L、(10.12±3.21)IU/L,差异均有统计学意义(P<0.05);两组女童的BAI、子宫容积和卵巢容积比较差异均无统计学意义(P>0.05)。结论中枢性性早熟女童的LH、LHRH水平明显高于外周性性早熟女童,能够通过LH、LHRH水平对两者进行区分。

LHRH固体脂质纳米粒口服给药系统的研究

目的考察以固体脂质纳米粒为载体包裹促黄体生成素释放激素的类似物(LHRH-A2)口服给药的可行性。方法采用溶剂扩散法制备LHRH-A2单硬脂酸甘油酯纳米粒(LHRH—A2 loaded monostearin solid lipid nanoparticles,LHRH-A2-MSLN),考察载药纳米粒的粒径、Zeta电位等理化性质;用HPLC测定药物的包封率及体外释放特性;以花(鱼骨)鱼(Hemibarbus maculates Bleeker)为模型动物,载药纳米粒经口灌给药后,分别测定鱼的受精率和催产率。结果LHRH-A2-MSLN的粒径为(284.1±103.6)nm,纳米粒Zeta电位为-(19.4±1.1)mV,HPLC测得药物包封率为63.4%。体外释放研究结果显示,LHRH-A2-MSLN在前8 h快速释放了纳米粒所载药物的26.8%,随后每天以1.9%的速率持续释放。体内药效学研究表明,50μg·kg-1剂量的LHRH-A2-MSLN 口灌给药后,平均催产率46.5%,受精率90.5%。结论用溶剂扩散法制备得到的LHRH-A2-MSLN具有一定的口服有效性。

LHRH类似物对体外培养肝癌细胞增殖阻抑作用的实验研究

目的 :探讨黄体素释放激素 (LHRH)类似物对肝癌细胞增殖的调节作用 ,为阐明LHRH在肝癌发病中的作用机制提供实验资料。 方法 :以体外培养的人肝癌细胞系hHCC和大鼠肝癌细胞系FSK 790 2为研究对象 ,用MTT试验检测LHRH类似物对这两种肝癌细胞生长的抑制作用 ;用流式细胞仪测定LHRH类似物作用后癌细胞的细胞周期变化 ;用免疫组化染色法检测PCNA和Bax蛋白表达以反映LHRH类似物对癌细胞增殖和程序性死亡指标的影响。 结果 :MTT试验表明 ,LHRH类似物可抑制hHCC和FSK 790 2的生长 ,并且这种作用呈时间和剂量依赖关系。LHRH类似物作用后 ,肝癌细胞中G1/G0 期细胞比率上升 ,S期细胞比率下降 ,说明细胞生长停滞。LHRH类似物可使癌细胞中PCNA免疫反应阳性细胞比率下降 (P <0 .0 5 ) ;而Bax阳性细胞比率增加 (P <0 .0 5 )。 结论 :LHRH类似物具有体外抑制肝癌细胞增殖的活性 ;

LHRHa靶向紫杉醇脂质体的制备及体外抗肿瘤作用

目的:制备促黄体激素释放激素类似物(Luteinizing hormone-releasing hormone analogues,LHRHa)靶向紫杉醇脂质体(Paclitaxel liposomes,PTX-Lipo),研究其在体外增强紫杉醇(Paclitaxel,PTX)对卵巢癌A2780/DDP细胞的抑制作用。方法:采用薄膜超声法制备PTX-Lipo与LHRHa靶向紫杉醇脂质体(LHRHa-Paclitaxel liposomes,LHRHa-PTX-Lipo),用透射电镜考察脂质体形态;高效液相色谱法测定2种PTX-Lipo的包封率;激光共聚焦法通过卵巢癌A2780/DDP细胞对4-氟-7-硝基-2,1,3-苯并氧杂恶二唑荧光素的摄取检测来反映细胞对NBD-Lipo与NBD-LHRHa-Lipo的摄取情况;MTT法及细胞克隆形成实验检测LHRHa-PTX-Lipo体外对卵巢癌细胞的生长抑制情况。结果:制备LHRHa-PTX-Lipo的平均粒径123.4 nm,包封率在90%以上;A2780/DDP细胞对NBD-LHRHa-Lipo组的荧光摄取明显高于NBD-Lipo组;LHRHa-PTX-Lipo对A2780/DDP细胞的生长及克隆形成抑制明显高于PTX组及PTX-Lipo组(P<0.05)。结论:采用薄膜超声法制备的LHRHa-PTX-Lipo可使药物在靶部位聚集,增强药物对卵巢癌细胞的抑制作用。