应用正交试验研究麻疹疫苗保护剂和冻干条件

对冻干麻疹活疫苗保护剂、冻干条件等多因素，分三个位级，运用正交实验设计进行试验，并初步筛选出各种保护剂最优成分及冻干过程中温度控制的一般要求。以冻干麻疹活疫苗试验为实例，介绍应用正交试验法在配比配方等多因素情况下的科学性和先进性。

人脂肪间充质干细胞条件培养基冻干粉促进皮肤成纤维细胞迁移、细胞外基质合成和抑制巨噬细胞炎症

目的探讨人脂肪间充质干细胞条件培养基冻干粉(hADMSCs-CMLP)对成纤维细胞(HFF-1)迁移、细胞外基质合成水平的影响,以及对小鼠巨噬细胞(Raw264.7)炎症因子释放的影响。方法收集人脂肪间充质干细胞P3代细胞条件培养基上清液,经冷冻干燥后,获得冻干粉制剂。使用前用去离子水溶解,添加到人成纤维细胞HFF-1和小鼠巨噬细胞Raw264.7培养基中。用细胞划痕实验筛选冻干粉的浓度,用活细胞工作站和transwell方法检测人成纤维细胞迁移和细胞增殖情况;qRT-PCR法检测成纤维细胞细胞外基质蛋白纤维粘连蛋白、弹性蛋白、I型胶原蛋白、MMP-1的mRNA水平变化;ELISA法测定巨噬细胞Raw264.7炎症因子TNF-α、IL-6释放情况。结果分离传代培养后,得到的P3代hADMSCs呈长梭形漩涡状并贴壁生长,有立体感,其间充质干细胞表面标志性抗原CD73、CD90、CD105阳性表达率均大于95.00%,CD34、CD45、HLA-DR均小于2.00%;诱导培养21~28 d后出现明显的成脂、成骨和成软骨细胞特性;细胞划痕实验显示50%的hADMSCs条件培养基冻干粉对成纤维细胞划痕修复效果最好。HFF-1细胞与hADMSCs条件培养基冻干粉共培养24 h,HFF-1细胞迁移率增加了近4倍(P<0.001);qRT-PCR结果显示,hADMSCs条件培养基冻干粉共培养处理48 h,HFF-1细胞纤维粘连蛋白、弹性蛋白、I型胶原蛋白基因表达相对于对照组分别上调了2.07倍(P<0.001)、3.92倍(P<0.001)和2.37倍(P<0.001),MMP-1基因表达水平显著降低了2.98倍(P<0.001);hADMSCs条件培养基冻干粉与LPS刺激的小鼠巨噬细胞(Raw264.7)共孵育24 h,与LPS组相比,TNF-α下降了20.7%(P<0.01),IL-6下降了83.9%(P<0.001)。结论hADMSCs条件培养基冻干粉能够显著促进成纤维细胞迁移,同时促进成纤维细胞的纤维粘连蛋白、弹性蛋白、I型胶原蛋白转录水平升高;hADMSCs条件培养基冻干粉还能显著抑制TNF-α和IL-6炎性因子的分泌。因此,hADMSCs条件培养基冻干粉在创伤修复、组织工程和美容抗衰领域具有一定应用潜力。

植物乳杆菌增殖培养及其浓缩型冻干发酵剂的制备

在发酵肉制品的发与应用生产中,浓缩型冻干发酵剂的制备具有重要的研究价值。该研究以植物乳杆菌为目标菌株,首先,研究不同生长因子对菌株的增殖作用,利用正交实验设计对生长因子进行复配,得到佳增殖培养条件;其次,研究离心条件在菌体富集时对菌体损失率和存活率的影响;后,研究冻干条件以及冻干保护剂选择对浓缩发酵剂菌粉成品特性的影响。结果表明,在MRS液体培养基内添加8%胡萝卜汁、8%番茄汁、0.75%CaCO3为佳增殖培养条件,活菌数达2.68×109CFU/mL;菌体佳富集条件为离心机转速4 000 r/min离心10 min,离心收得率达到96.87%;佳冻干条件是作为悬浮基质的脱脂乳浓度为10%,冻干厚度为0.5cm,冻干保护剂组合为：海藻糖（10%）、麦芽糖（12%）、谷氨酸钠（8%）,此条件下活菌数为3.71×109CFU/mL,菌体存活率达到75.43%;菌体冻干36 h后,其水分含量可满足储藏要求（1.5%~3.0%）。

Optimization of Protectant, Salinity and Freezing Condition for Freeze-Drying Preservation of Edwardsiella tarda

Novel preservation condition without ultra-low temperature is needed for the study of pathogen in marine fishes. Freeze-drying is such a method usually used for preservation of terrigenous bacteria. However, studies using freeze-drying method to preserving marine microorganisms remain very limited. In this study, we optimized the composition of protectants during the freeze-drying of Edwardsiella tarda, a fish pathogen that causes systemic infection in marine fishes. We found that the optimal composition of protectant mixture contained trehalose(8.0%), skim milk(12.0%), sodium citrate(2.0%), serum(12.0%) and PVP(2.0%). Orthogonal and interaction analyses demonstrated the interaction between serum and skim milk or sodium citrate. The highest survival rate of E. tarda was observed when the concentration of Na Cl was 10.0, 30.0 and between 5.0 and 10.0 g L^(-1) for preparing TSB medium, E. tarda suspension and protectant mixture, respectively. When E. tarda was frozen at-80℃ or-40℃ for 6 h, its survival rate was higher than that under other tested conditions. Under the optimized conditions, when the protectant mixture was used during freeze-drying process, the survival rate(79.63%–82.30%) of E. tarda was significantly higher than that obtained using single protectant. Scanning electron microscopy(SEM) image indicated that E. tarda was embedded in thick matrix with detectable aggregation. In sum, the protectant mixture may be used as a novel cryoprotective additive for E. tarda.

水溶性甘草次酸冻干粉的制备及理化分析

目的:制备水溶性甘草次酸冻干粉,并进行理化分析。方法:将甘草次酸溶解于三氯甲烷和乙醇的混合溶剂作为油相,甘露醇溶解于三氯甲烷饱和水溶液作为水相,使用高速匀浆器进行乳化形成油包水型(o/w)粗乳,接着转入高压均质机内乳化得到亚微乳。再利用真空旋转蒸发除去有机溶剂,经冷冻干燥获得水溶性甘草次酸冻干粉。形成粗乳的第一步乳化工艺借助单因素法进行优化。结果:甘草次酸粗乳的最佳制备工艺条件是油相和水相体积比为15%,甘草次酸浓度为155 mg·mL^(-1),乳化次数为18次;水溶性甘草次酸冻干粉在水中分散良好呈现乳光,没有肉眼可见颗粒;其平均粒径为241.1 nm,扫描电镜下观察呈规则棒状;在37℃水中溶解度为23.08μg·mL^(-1),比甘草次酸原粉(3.84μg·mL^(-1))提高了大约5倍。结论:乳化法能将甘草次酸粒径减小至纳米范畴,并且提高其水中溶解度。

植物乳杆菌真空冷冻干燥工艺的优化

采用真空冷冻干燥法,在高密度培养、离心制备菌泥的基础上,通过正交试验,优化植物乳杆菌冻干保护剂及冻干条件,研究不同条件下的菌体存活率。结果表明:植物乳杆菌的最佳冻干保护剂为低聚果糖5 g/100 mL、脱脂乳粉12.5 g/100 mL、半乳糖4.5 g/100 mL、乳糖3 g/100 mL、脯氨酸2.5 g/100 mL、水溶性海藻糖3 g/100 mL;最佳冻干条件为菌泥比例50 g/100 mL、预冻温度-45℃、预冻时间4 h、冻干厚度1.0 cm、真空度0.2 mbar。此条件下制备的植物乳杆菌冻干粉菌体存活率为88.74%。