葡萄内脂对PC12神经细胞损伤的保护作用研究

目的探讨葡萄内脂对过氧化氢(H2O2)诱导的肾上腺嗜铬瘤细胞(PC12)神经细胞损伤的保护作用。方法体外培养PC12细胞,建立PC12细胞过氧化氢损伤模型。将处于对数生长期的PC12细胞分为正常对照组、模型组、阳性对照组、5μmol/L葡萄内脂组、25μmol/L葡萄内脂组、50μmol/L葡萄内脂组。采用不同浓度(5μm/L,25μm/L和50μm/L)葡萄内脂对PC12细胞进行干预,通过测定细胞存活率、细胞上清液中乳酸脱氢酶水平和细胞内氧化活性物质(ROS)水平评价干预效果。结果模型组PC12细胞存活率显著低于正常对照组及阳性对照组; 25μmol/L、和50μmol/L葡萄内脂组PC12细胞存活率(与阳性对照组相当)显著高于模型组,随着葡萄内脂浓度的增加,H2O2诱导损伤的PC12细胞的存活率呈升高趋势,组间比较差异有统计学意义(P <0. 05)。模型组PC12细胞上清液乳酸脱氢酶水平明显高于正常组及阳性对照组,5μmol/L、25μmol/L和50μmol/L葡萄内脂组细胞上清液乳酸脱氢酶水平(与阳性对照组相当)均显著低于模型组,且随着葡萄内脂浓度的增加,乳酸脱氢酶水平呈降低趋势,组间比较差异有统计学意义(P <0. 05)。模型组PC12细胞ROS水平显著高于正常对照组及阳性对照组,5μmol/L、25μmol/L和50μmol/L葡萄内脂组PC12细胞ROS水平(与阳性对照组相当)均显著低于模型组,且随着葡萄内脂浓度的增加,ROS水平呈降低趋势,差异有统计学意义(P <0. 05)。结论葡萄内脂对H2O2诱导损伤的PC12神经细胞具有明显的保护作用,可能与其能维持细胞膜的完整性、发挥抗氧化作用有关。

葡萄糖酸内脂在肉类工业中的应用

1 前言 葡萄糖酸-δ-内脂(Glucono-dlta-lactone),本文简称GdI是葡萄糖酸的中性内脂,在水溶液中水解形成葡萄糖酸。它是果汁、果酒、麦芽及啤酒中存在的天然成分,并且是碳水化合物新陈代谢的中间产物,所以对人体无害。

葡萄糖酸δ内脂在镍的化学退除中的缓蚀作用

本文探讨了在铁基上的Ｎｉ／Ｎｉ镀层在以硝基芳香族化合物为氧化剂的碱性退除液中的退除速率、腐蚀速率，发现葡萄糖酸δ内脂在退除液中有较好的缓蚀作用，所筛选的退除配方适于铁基精细镍镀件的退除．

安徽郎溪成为我国最大葡萄糖酸内脂生产基地

目前，安徽省郎溪县依托东兴食品和兴宙医药两家企业，年生产葡萄糖酸内脂的能力达7000吨，已占据国内同类产品75％的市场，成为我国最大的葡萄糖酸内脂生产供应基地。

葡萄糖醛酸内酯制备和表征研究

针对葡萄糖醛酸内酯的制备问题,研究提出了一种新的葡萄糖醛酸内酯制备及纯化方法,研究表明:在对葡萄糖醛酸内酯物品进行纯化的过程中,以甲醇和去离子水作为传话的流动相,然后使用C18反向键胶柱对其进行梯度洗脱,通过该种技术进行纯化以后,葡萄糖醛酸内酯的产率可以达到14.17%,纯度可以达到91.6%,通过显色实验分析、物理分析、红外分析、核磁共振分析以及色谱分析可以发现,该研究所制备的样品确定为葡萄糖醛酸内酯,且纯度相对较好。

促凝剂及小分子表面活性剂对大豆分离蛋白乳状液凝胶性质的影响

大豆分离蛋白乳状液凝胶在豆制品以及肉制品中有广泛的应用,因此如何提升乳状液凝胶的强度和持水性受到广泛关注。作者利用流变、质构和显微结构分析,详细研究了促凝剂、乳状液稳定性、小分子表面活性剂对于大豆分离蛋白乳状液凝胶强度和持水性的影响。结果表明,乳状液稳定性好的其凝胶强度与持水性也相对要好。对于促凝剂,硫酸钙与葡萄糖酸内脂混合凝胶要优于两者单独促凝的效果。当吐温20添加量小于体积分数0.4%时,其能够减弱凝胶强度,体积分数高于0.4%时,能够增强凝胶强度,但是持水性都是呈下降趋势。大豆卵磷脂对于凝胶强度没有明显的改善,但是对于持水性有明显的提高作用。

碳源对Li3V2（PO4）3/C正极材料电化学性能的影响

碳源是影响聚阴离子型锂离子电池正极材料电化学性能的关键因素之一.研究碳源对Li3V2(PO4)3正极材料晶体结构、形貌、颗粒尺寸、热解碳形态、导电性和电化学性能的影响.分别以聚丙烯腈、丹宁酸、没食子酸、葡萄糖酸内脂为碳源,通过碳热还原法制备Li3V2(PO4)3/C复合正极材料.结果表明,相比聚丙烯腈、丹宁酸,没食子酸、葡萄糖酸内脂为碳源制备的Li3V2(PO4)3/C具有更高的电化学活性和循环稳定性.在20 C的高倍率下,以葡萄糖酸内脂为碳源制备的Li3V2(PO4)3/C表现出最高的放电容量,这主要归于材料高的结晶度、导电性以及材料颗粒表面完整的包覆碳层.

安徽朗溪成为我国最大葡萄糖酸内脂生产基地

目前，安徽省朗溪县依托东兴食品和兴宙医药两家企业，年生产葡萄糖酸内脂的能力达7000吨，已占据国内同类产品75％的市场，成为我国最大的葡萄糖酸内脂生产供应基地。

Inhibitive effects of glucose and free fatty acids on proliferation of humanvascular endothelial cells in vitro

OBJECTIVES: To investigate the effects of glucose and free fatty acids (FFAs) on the proliferation and cell cycle of human vascular endothelial cells in vitro, and to examine whether the combined presence of elevated FFAs and glucose may cross-amplify their individual injurious effects. METHODS: Cultured human vascular endothelial cells (ECV304) were incubated with various concentrations of glucose and/or FFAs (palmitate and/or oleate) for 24 - 96 h. Morphologic alterations were observed using a phase contrast microscope and an electron microscope. Inhibition of proliferation was measured by a colorimetric 3-[4, 5-dimethyl thiazol-2-yl]-2, 5-diphenyltetrazolium bromide (MTT) assay. Cell viability was determined using trypan blue exclusion. Distribution of cells along phases of the cell cycle was analyzed by flow cytometry. RESULTS: Glucose 15 or 30 mmol/L, palmitate (PA) 0.25 or 0.5 mmol/L, and oleate (OA) 0.5 mmol/L inhibited proliferation and accelerated death of endothelial cells in a dose-and-time-dependent manner. After treatment with elevated glucose and/or FFAs, the G(0)/G(1) phase cells increased, whereas S phase cells decreased, suggesting that high glucose and/or FFAs mainly arrested endothelial cells at G(0)/G(1) phase. The inhibitive rates of proliferation and population of dead cells in endothelial cells incubated with glucose plus FFAs (glucose 30 mmol/L + PA 0.25 mmol/L, glucose 30 mmol/L + OA 0.5 mmol/L, glucose 30 mmol/L + PA 0.25 mmol/L + OA 0.5 mmol/L) increased more markedly than those treated with high glucose or FFAs (PA and/or OA) alone. CONCLUSION: Both high ambient glucose and FFAs can inhibit proliferation and accelerate death of endothelial cells in vitro. These changes were cross-amplified in the combined presence of high levels of glucose and FFAs.

Inhibitive effects of glucose and free fatty acids on proliferation of human vascular endothelial cells in vitro

s To investigate the effects of glucose and free fatty acids (FFAs) on the proliferation and cell cycle of human vascular endothelial cells in vitro , and to examine whether the combined presence of elevated FFAs and glucose may cross amplify their individual injurious effects Methods Cultured human vascular endothelial cells (ECV304) were incubated with various concentrations of glucose and/or FFAs (palmitate and/or oleate) for 24-96 h Morphologic alterations were observed using a phase contrast microscope and an electron microscope Inhibition of proliferation was measured by a colorimetric 3 [4, 5 dimethyl thiazol 2 yl] 2, 5 diphenyltetrazolium bromide (MTT) assay Cell viability was determined using trypan blue exclusion Distribution of cells along phases of the cell cycle was analyzed by flow cytometry Results Glucose 15 or 30 mmol/L, palmitate (PA) 0 25 or 0 5 mmol/L, and oleate (OA) 0 5 mmol/L inhibited proliferation and accelerated death of endothelial cells in a dose and time dependent manner After treatment with elevated glucose and/or FFAs, the G 0/G 1 phase cells increased, whereas S phase cells decreased, suggesting that high glucose and/or FFAs mainly arrested endothelial cells at G 0/G 1 phase The inhibitive rates of proliferation and population of dead cells in endothelial cells incubated with glucose plus FFAs (glucose 30 mmol/L+PA 0 25 mmol/L, glucose 30 mmol/L+OA 0 5 mmol/L, glucose 30 mmol/L+PA 0 25 mmol/L+OA 0 5 mmol/L) increased more markedly than those treated with high glucose or FFAs (PA and/or OA) alone Conclusion Both high ambient glucose and FFAs can inhibit proliferation and accelerate death of endothelial cells in vitro These changes were cross amplified in the combined presence of high levels of glucose and FFAs