PLGA/O-CMC载药纳米粒子的体外释药行为研究

本文以聚乳酸_乙醇酸共聚物 (PLGA)和自行制备的O_羧甲基壳聚糖 (O_CMC)为原料 ,以5_氟尿嘧啶 (5_FU)为抗癌药物模型 ,采用自身设计的改良复乳法制备了载药纳米微粒。微粒平均粒径为 98 5nm ,粒径分布指数为 0 192 ,粒子表面 ξ电位为 6 1 4 8eV ,载药率高达 18 9% ,包封率为86 %。然后用SEM动态监测载药纳米粒子降解过程中表面形貌的变化 ,并连续追踪粒子降解过程中的质量损失和降解介质的pH变化。载药纳米粒子在PBS中的释药行为研究表明 :(1)前 12h的释药动力学符合Huguchi方程 ,具有一级释放特性 ;(2 )在 2

PLGA/O-CMC载药纳米微粒的体外降解及释药行为研究

本研究以聚乳酸乙醇酸共聚物(PLGA)和自行制备的O羧甲基壳聚糖(OCMC)为原料,以5氟尿嘧啶(5FU)为抗癌药物模型,采用自身设计的改良复乳法制备了载药纳米微粒。微粒平均粒径为98.5nm,粒径分布指数为0.192,粒子表面ξ电位为61.48eV,载药率高达18.9%。然后用SEM动态监测载药纳米粒子降解过程中表面形貌的变化,并连续追踪粒子降解过程中的质量损失和降解介质的pH变化。载药纳米粒子在PBS中的释药行为研究表明,(1)前12h的释药动力学符合Huguchi方程,具有一级释放特性;(2)在20d内的释药动力学符合零级释放特性。细胞凋亡实验结果表明载药纳米粒子对TJ905脑胶质瘤细胞增殖有明显的抑制作用。

丁香苦苷单体与丁香苦苷PEG-PLGA纳米粒在大鼠体内药动学比较研究

目的：通过测定大鼠血浆中丁香苦苷的含量,对具有抗乙肝病毒的丁香苦苷单体和丁香苦苷PEG-PLGA纳米粒进行大鼠体内药动学比较研究。方法：Wistar大鼠尾静脉注射（40g/L）给予丁香苦苷和丁香苦苷PEG-PLGA-NPs后,HPLC法测定不同时间点测定血浆中的药物浓度,所得数据用3p97软件分析求算药动学参数。结果：丁香苦苷浓度在0.01~100.30μg/L范围内线性关系良好,回归方程为Y=13250X＋16364,提取回收率在85%以上、RSD低于5%。药动学参数表明丁香苦苷单体与丁香苦苷PEG-PLGA-NPs在大鼠体内过程均符合二室模型,丁香苦苷PEG-PLGA溶液的T1/2α和T1/2β是丁香苦苷溶液的1.58倍和11.46倍,AUC是丁香苦苷溶液的2.40倍,血浆清除率约为其0.42倍。结论：本实验研究数据为进一步研究丁香苦苷的临床应用提供了重要的实验数据。

共载TPE衍生物和纳米银的PLGA复合载药体系的抑菌活性研究

通过复乳法合成复合纳米载药体系PLGA@TPE@Ag,其粒径大小300 nm左右,分散均一。其载药量达到了35±3.7%,包封率为73±0.9%,具有明显的药物缓释特性。PLGA@TPE@Ag对耐药性的大肠杆菌MIC值是2.3±0.09μg/mL。PLGA@TPE@Ag质量浓度为20μg/mL时对金黄色葡萄球菌和大肠杆菌的抑制率都高达90%以上。载药体系PLGA@TPE@Ag对细菌细胞内部形态的破坏可能是导致其细菌被抑制存活的主要机制。小鼠器官毒性试验明确PLGA@TPE@Ag无毒性。复合载药体系的抑菌活性相对于单一的载药体系有极大的提高。

The studies of PLGA nanoparticles loading atorvastatin calcium for oral administration in vitro and in vivo

A biodegradable poly(lactic-co-glycolic acid) loading atorvastatin calcium(AC) nanoparticles(AC-PLGA-NPs) were prepared by probe ultrasonication and evaporation method aiming at improving the oral bioavailability of AC. The effects of experimental parameters, including stabilizer species, stabilizer concentration and pH of aqueous phase, on particle size were also evaluated. The resultant nanoparticles were in spherical shape with an average diameter of 174.7 nm and a narrow particle size distribution. And the drug loading and encapsulation efficiency were about 8% and 71%, respectively. The particle size and polydispersion were almost unchanged in 10 days. The release curves of AC-PLGA-NPs in vitro displaying sustained release characteristics indicated that its release mechanisms were matrix erosion and diffusion. The pharmacokinetic study in vivo revealed that the Cmax and AUC0-∞ of AC-PLGA-NPs in rats were nearly 3.7-fold and 4.7-fold higher than that of pure atorvastatin calcium suspension. Our results demonstrated that the delivery of AC-PLGANPs could be a promising approach for the oral delivery of AC for enhanced bioavailability.

荆芥内酯聚乳酸乙醇酸纳米粒的制备及其稳定性研究

目的制备荆芥内酯聚乳酸乙醇酸纳米粒,并优化其制备工艺。方法以粒径、分散度、包封率和载药量为指标,对溶剂挥发法、溶剂扩散法和溶剂-非溶剂法制备荆芥内酯纳米粒进行比较。在单因素考察基础上,采用正交设计法对纳米粒的处方和溶剂-非溶剂法制备工艺进行优化,并考察了4℃和25℃条件下纳米粒溶液的稳定性。结果溶剂-非溶剂法制备的荆芥内酯纳米粒形态圆整,大小均匀,平均粒径(80.3±1.75)nm,分散度0.0144±0.00625,包封率可达52.53%±0.97%,载药量27.56%±0.91%,显著优于溶剂挥发法和溶剂扩散法,且具有良好的稳定性。结论溶剂-非溶剂法制备荆芥内酯纳米粒具有工艺简便,粒径和分散度小,包封率和载药量高,重复性好,质量稳定的优点。

Insight into the preformed albumin corona on in vitro and in vivo performances of albumin-selective nanoparticles

Preformed albumin corona of albumin-nonselective nanoparticles(NPs)is widely exploited to inhibit the unavoidable protein adsorption upon intravenous administration.However,very few studies have concerned the preformed albumin corona of albumin-selective NPs.Herein,we report a novel type of albumin-selective NPs by decorating 6-maleimidocaproyl polyethylene glycol stearate(SA)onto PLGA NPs(SP NPs)surface,taking albuminnonselective PLGA NPs as control.PLGA NPs and SP NPs were prepared by emulsion-solvent evaporation method and the resultant NPs were in spherical shape with an average diameter around 180 nm.The corresponding albumin-coating PLGA NPs(PLGA@BSA NPs)and albumin-coating SP NPs(SP@BSA NPs)were formulated by incubating SP NPs or PLGA NPs with bovine serum albumin solution,respectively.The impact of albumin corona on particle characteristics,stability,photothermal effect,cytotoxicity,cell uptake,spheroid penetration and pharmacokinetics was investigated.In line with previous findings of preformed albumin coating,PLGA@BSA NPs exhibited higher stability,cytotoxicity,cell internalization and spheroid penetration performances in vitro,and longer blood circulation time in vivo than those of albumin-nonselective PLGA NPs,but albumin-selective SP NPs is capable of achieving a comparable in vitro and in vivo performances with both SP@BSA NPs and PLGA@BSA NPs.Our results demonstrate that SA decorated albumin-selective NPs pave a versatile avenue for optimizing nanoparticulate delivery without preformed albumin corona.

载基因/化疗药物双层纳米粒的制备及其体内外抗乳腺癌效应初步研究

目的以血管生成为靶点治疗肿瘤的假说验证后,抗肿瘤血管生成基因治疗因其明显的优势而受到关注,与化疗联合,既抑制肿瘤血管内皮细胞,亦杀灭肿瘤细胞,协同增强抗肿瘤效应。文中探讨了共载血管内皮生长因子(VEGF)的小型干扰RNA(siRNA)与化疗药物(EPI)的双层纳米粒的负载基因能力和体内外抑制乳腺癌初步效应。方法将合成的mPEG-g-CS与PLGA纳米粒通过超声透析法制备成双层纳米粒(DL NPs),外层为mPEG-g-CS,负载siRNA,内层为PLGA纳米粒,包载化疗药物EPI,研究双层纳米粒的理化性质,基因负载能力。将裸鼠随机数字表法分成4组,每组6只,重复3次:等渗盐水组,游离EPI组、mPEG-g-CS-siRNA NPs组以及DL NPs-siRNA组,EPI给药剂量为25 mg EPI/kg,mPEG-g-CS-siRNA以及DL-siRNA NPs给药剂量为65μg siRNA/kg,开始进行治疗。定期测量肿瘤长宽,22 d时处死裸鼠,取出肿瘤组织、称重。结果琼脂糖凝胶电泳阻滞实验表明mPEG-g-CS能有效地与pDNA结合形成稳定的复合物,且对细胞活性影响小,证明其可作为基因载体。siRNA浓度为100 nmol/L为最佳负载浓度。当N/P比例为5时,mPEG-g-CS-siRNA的粒径最小[(-12.70±0.42)nm],而对DL NPs-siRNA而言,当N/P比例为20时其粒径最小[(153.82±30.15)nm]。当N/P比例为0.1时,可以看到有少量的pDNA迁移,此时mPEG-g-CS不能完全缩合pDNA;当N/P比例为0.4及之上,pDNA完全被mPEG-g-CS阻滞,此时mPEG-g-CS已经完全缩合pDNA。以聚乙烯亚胺(PEI)为阳性对照,MCF-7细胞、HUVEC细胞与纳米粒共孵育24、48、72 h后,mPEG-g-CS-p DNA NPs都显示出较低的毒性。但是随着培养时间的延长,mPEG-g-CS-p DNA NPs的毒性增加。siRNA浓度为100 nmol/L时,MCF-7细胞存活率为78.66%,HUVEC的细胞存活率为85.69%,毒性更大。在孵育24 h时,DL NPs-siRNA浓度为0.5、50和500μg/mL时MCF-7细胞的平均存活率分别是92.4%、78.1%和51.4%,并且,随着孵育时间的延长,各组细胞存活率均降低。治疗22 d后,游离EPI组的肿瘤抑制率约为22.36%,mPEG-g-CS-siRNA组的肿瘤抑制率约为85.01%,相比之下,DL NPs-siRNA组肿瘤抑制率高达99.90%。22 d后,解剖小鼠,取出肿瘤组织,对照组的肿瘤体积和质量最大,DL NPs-siRNA组最小,肿瘤几乎完全消失。结论DL NPs可用于负载siRNA及化疗药物,有望成为一种新的抗肿瘤药物输送体系。

红细胞膜包裹PLGA纳米粒的制备和体外毒性及药物释放初探

目的:制备红细胞膜包裹PLGA纳米粒(RBC-NP)并进行结构表征、稳定性及体外毒性和药物释放的探究。方法:纳米沉淀法制备PLGA纳米粒(PLGA NP);脂质体挤压法制备红细胞膜和RBC-NP;Malvern ZS90测定粒径和分散系数;透射电镜(TEM)观察RBC-NP的形态。将DiOC18(3)载入RBC-NP和PLGA NP,探究二者的药物体外释放特性。采用CCK8法检测细胞的相对增殖率,比较RBC-NP与PLGA NP的细胞毒性。结果:RBC-NP与PLGA NP的粒径之差为11.1~14.2 nm,分散系数在0.131~0.155。TEM显示RBC-NP呈壳-核结构,核心为PLGA,外包裹单层红细胞膜。RBC-NP在PBS和超纯水中6 d内均保持稳定。RBC-NP具有良好体外缓释作用。0.25,0.5,1 mg·m L^(-1)3组中,RBC-NP的细胞相对增殖率均显著性高于PLGA NP(P<0.01)。结论:具有壳-核结构的RBC-NP已被成功制备,具有药物缓释作用且体外毒性显著降低。

两种克班宁长循环纳米粒的急性毒性与抗心律失常作用研究

目的对两种经PEG修饰载体材料(PELGE、PLGA)制备的克班宁(Crebanine,Cre)长循环纳米粒(PELGE-Cre-NPs、PLGA-Cre-NPs)进行急性毒性试验与抗心律失常作用研究,探讨其增效减毒的效果。方法采用Bliss法对PELGE-Cre-NPs与PLGA-Cre-NPs进行小鼠急性毒性试验,求半数致死量(LD_(50));采用氯仿诱发小鼠心室纤颤模型、氯化钡(BaCl_(2))及乌头碱致心律失常大鼠模型对两种纳米粒进行药效作用考察。结果PLGA-Cre-NPs与PELGE-Cre-NPs静脉注射的LD_(50)分别为13.619 mg·kg^(-1)与14.839 mg·kg^(-1),均比克班宁静脉注射的LD_(50)(9.382 mg·kg^(-1))明显增加。与模型对照组比较,两种纳米粒均能明显对抗氯仿诱发的小鼠心室纤颤、对抗氯化钡诱导的大鼠心律失常,明显提高乌头碱诱发大鼠室性早搏(VPB)、室性心动过速(VT)、心室纤颤(VF)及心脏停搏(CA)的阈剂量(P<0.05,P<0.01,P<0.001)。与克班宁(5 mg·kg^(-1))实验组比较,PELGE-Cre-NPs高剂量(5 mg·kg^(-1))组恢复窦性心律维持时间≥5 min的鼠数量明显增多(P<0.05),心脏停搏乌头碱阈剂量明显提高(P<0.05)。结论两种材料纳米粒PLGA-Cre-NPs与PELGE-Cre-NPs的毒性较克班宁小,并具有较明显的抗心律失常活性,且作用效果强于游离克班宁,达到增效减毒作用。

荆芥内酯纳米粒冻干粉末的制备工艺及质量研究

目的制备荆芥内酯聚乳酸乙醇酸纳米粒冻干粉末,并探讨其工艺与质量评价标准。方法以外观、色泽、再分散性为指标,优选支架剂的种类和浓度及冻干工艺;并对该冻干粉末的外观、再分散性、pH值、纳米粒的形态、粒径分布、多分散系数、质量分数、包封率及载药量等质量评价指标进行考察。结果10%甘露醇作为支架剂可以较好地防止纳米粒的聚集,优化的冻干工艺为-45℃预冻10 h,升温至-25℃维持5 h,再升温至-5℃维持2 h,再升温至10℃维持2 h,最后升温至30℃维持6 h。冻干粉末的外观和分散性良好,平均pH值为6.25,纳米粒平均粒径为80.2 nm,多分散系数为0.024 8,包封率为52.17%,载药量为28.73%。结论荆芥内酯纳米粒冻干粉末制备工艺简便、重复性好;所选用的质量评价方法适用于该冻干粉末,可有效反映其性质。

Layer by layer surface engineering of poly (lactide-co-glycolide) nanoparticles:A versatile tool for nanoparticle engineering for targeted drug delivery

Recent work regarding the Layer by Layer (LbL) engineering of poly(lactide-co-glycolide) nanoparticles (PLGA NPs) is reviewed here.The LbL engineering of PLGA NPs is applied as a means of generating advanced drug delivery devices with tailored recognition,protection,cargo and release properties.LbL in combination with covalent chemistry is used to attach PEG and folic acid to control cell uptake and direct it towards cancer cells.LbL coatings composed of chitosan and alginate show low protein interactions and can be used as an alternative to Pegylation.The assembly on top of LbL coatings of lipid layers composed of variable percentages of 1,2-dioleoyl-sn-glycero-3-choline (DOPC) and 1,2-dioleoyl-sn-glycero-3-phosphoL-serine (DOPS) increases NP uptake and directs the NPs towards the endoplasmic reticulum.The antibody anti-TNF-α is encapsulated forming a complex with alginate that is assembled LbL on top of PLGA NPs.The antibody is released in cell culture following first order kinetics.The release kinetics of encapsulated molecules inside PLGA NPs are studied when the PLGA NPs are coated via LbL with different polyelectrolytes.The intracellular release of encapsulated Doxorubicin is studied in the HepG2 cell line by means of Fluorescence Lifetime Imaging.