利用CO_2培养箱敞开式不换液羊水细胞培养方法的改进

本文对羊水培养方法进行了改进研究,探讨了培养液 pH 值对羊水细胞生长的影响。结果表明用 CO_2培养箱敞开培养,在 CO_2浓度为5.4%时羊水细胞最容易贴壁生长,一次性加液中间不换液可保持细胞生长的微环境稳定,是羊水细胞培养成功的关键。     

pH指示剂吸收度比值法测定盐酸乙胺丁醇的含量

本文报道pH指示剂吸收度比值法测定盐酸乙胺丁醇的含量。该法采用指示剂为0.05%茜素黄R,测定波长374nm和500nm;标准液为0.1mol/L NaOH;仪器为WFZ-800D_2型分光光度计。测得三批盐酸乙胺丁醇的含量分别为99.5±0.04%,99.4±0.05%和99.6±0.03%.同时与药典法比较,结果一致。     

强酸和强碱中和过程的PH控制

讨论了强酸、强碱中和过程ＰＨ控制方案。以０．９ｍｏｌ／Ｌ的ＮａｏＨ中和０．９ｍｏｌ／Ｌ的ＨＮＯ３，流量增量为０．１－０．３ｋｇ／ｍｉｎ，用模糊控制将ＰＨ控制在各要求的值上，ΔｐＨ≤０．２，获得满意的结果。     

动物细胞培养过程中pH和溶氧的关联控制

本文通过对动物细胞培养过程中pH值和溶氧(DO)水平控制要求的分析,设计了用空气、氧气、氮气和二氮化碳四组气体关联控制pH值和DO水平的控制系统。该系统根据对瞬时pH值和DO值参数的检测,通过微处理机进行一系列的逻辑判断和具有PI调节规律的DDC增量词节计算,再经四气体关联互补计算和多重时序控制环节,综合调节四组气体电磁阀的相互开闭时间,实现对培养过程中pH值和DO水平的控制,满足动物细胞生长的需要。     

Oxidative stress induced by iron released from transferrin in low pH peritoneal dialysis solution

Background. Transferrin binds extracellular iron and protectstissues from iron-induced oxidative stress. The binding of ironand transferrin is pH dependent and conventional peritonealdialysis (PD) solutions have unphysiologically low pH values.Herein, we investigated whether conventional PD solution releasesiron from transferrin and if the released iron causes oxidativestress. Methods. Effects of PD solutions on iron binding to transferrinwere examined with purified human transferrin and transferrinin dialysates drained from PD patients. Oxidative stress inducedby iron released from transferrin was evaluated in terms ofthe formation of thiobarbituric acid reactive substance (TBARS)and protein carbonylation in the human red blood cell (RBC)membrane. The iron deposition in peritoneal tissue from PD patientswas evaluated by Perls' staining with diaminobenzidine intensification. Results. Low pH PD solution released iron from transferrin.This iron release occurred within 1 min. Iron release was notobserved in neutralized PD solution. Iron released from transferrinin low pH PD solution increased TBARS formation and proteincarbonylation in the human RBC membrane. Iron deposition, whichis prominent in the fibrotic area facing the peritoneal cavity,was observed in the peritoneum of PD patients. Conclusions. Iron released from transferrin in low pH PD solutioncan produce oxidative stress in the peritoneum of a PD patient.Neutralizing PD solution can avoid this problem. Iron depositionin the peritoneum may participate in the pathogenesis of peritonealfibrosis in PD patients.     

大黄对兔内毒素性急性肺损伤胃肠粘膜pH值的影响

目的　研究大黄对兔内毒素性急性肺损伤 (ALI)胃肠粘膜 pH值 (i pH)的影响。 方法　 12只雄性新西兰兔 ,体重为 2 0～ 2 5kg ,随机分为生理盐水对照组 (CON组 ,n =6 )和内毒素组(LPS组 ,n =6 ) ,静注内毒素复制ALI模型。动物在注入LPS后 (2 0 5± 1 0 5 )h ,氧合指数 (PaO2 /FIO2 )≤ 30 0。此时为ALI,肺组织学可见肺泡水肿 ,肺泡壁淤血 ,肺泡内可见中性粒细胞浸润。另取12只雄性新西兰兔 ,待ALI模型成功 ,动物随机分为两组 :大黄组 (D组 ,n =6 )和对照组 (NS组 ,n =6 )。D组从胃管内注入大黄 2 0g/kg ,NS组从胃管中注入生理盐水 2 0 g/kg ,作为对照。观察各时点i pH的变化 (时点分为 :基础值时、ALI时、ALI后 1、2、3、4、5及 6h)。 结果　NS组i pH在ALI后 4、5及 6h较基础值时降低 (P <0 0 5 ) ,在ALI后 5h及 6h较ALI时降低 (P <0 0 5 ) ;D组i pH在ALI后 4h及 5h较NS组升高 (P <0 0 5 ) ,而在ALI后 6h较NS组同时点显著升高 (P <0 0 1)。结论　大黄可提高LPS性兔ALI胃肠粘膜pH值 ,因而对兔胃肠粘膜有保护作用     

长链核酸扩增技术评价病毒灭活效果的研究

目的:探讨用长链核酸扩增技术评价病毒灭活效果的可行性.方法:针对伪狂犬病毒(pseudorabies virus,PRV)糖蛋白gD基因前后的保守区设计预计产物长短不一的5对引物,用半巢式PCR技术扩增经低pH法(4.0±0.1)、巴氏消毒法[(60±1.0)℃]和s/D法(有机溶剂/洗涤荆)处理后的PRV核酸,同时以细胞感染法做平行对照.结果:低pH对PRV核酸有破坏作用,处理时间越长,核酸损伤程度越明显,处理60 min时,6.62 lgTCID50的PRV完全被灭活.5条不同长度PCR扩增产物中,只有3.9 kb的长片段检出与细胞培养结果一致.7.25 lgTCID50的PRV经(60±1.0)℃处理20 min后即被完全灭活,7.13 lgTCID50的PRV经s/D法处理1 h后被完全灭活,但各长度核酸片段扩增均为阳性,与细胞感染试验结果不符.结论:低pH对PRV核酸的损伤程度随处理时间的延长而增加;用长链PCR(3.9 kb)技术来评价经低pH法灭活病毒的效果是可行的,而该法不适合评价巴氏消毒法和S/D法灭活病毒的效果.     

Expression of Na+/HCO3− co‐transporter proteins (NBCs) in rat and human skeletal muscle

Aim: Sodium/bicarbonate co‐transport (NBC) has been suggested to have a role in muscle pH regulation. We investigated the presence of NBC proteins in rat and human muscle samples and the fibre type distribution of the identified NBCs. Methods and results: Western blotting of muscle homogenates and sarcolemmal membranes (sarcolemmal giant vesicles) were used to screen for the presence of NBCs. Immunohistochemistry was used for the subcellular localization. The functional test revealed that approximately half of the pH recovery in sarcolemmal vesicles produced from rat muscle is mediated by bicarbonate‐dependent transport. This indicates that the NBCs are preserved in the vesicles. The western blotting experiments demonstrated the existence of at least two NBC proteins in skeletal muscle. One NBC protein (approximately 150 kDa) seems to be related to the kidney/pancreas/heart isoform NBC1, whereas the other protein (approximately 200 kDa) is related to the NBC4 isoform. The two NBC proteins represent the electrogenic isoforms named NBCe1 and NBCe2. Membrane fractionation and immunofluorescence techniques confirmed that the two NBCs are located in the sarcolemmal membrane as well as in some internal membranes, probably the T‐tubules. The two NBCs localized in muscle have distinct fibre type distributions. Conclusions: Skeletal muscle possesses two variants of the sodium/bicarbonate co‐transporter (NBC) isoforms, which have been called NBCe1 and NBCe2.     

植入后全胚胎培养的培养基pH值改变对大鼠胚胎生长发育的影响

目的　探讨植入后全胚胎培养培养基最适pH值。方法　分离 9.5天龄Wistar大鼠胚胎 ,分别在实验组 (即不同pH :5 .5 ,6 .0 ,6 .5 ,7.0 ,7.5 ,8.0 ,8.5 ,9.0 )和对照组 (pH为 8.2 )的培养基 (1 0 0 %大鼠即刻离心血清 )中体外旋转培养4 8小时 ,观察pH值的改变对胚胎生长发育的影响。结果　与对照组比较 ,当培养基pH为 6 .5、6 .0和 9.0时培养胚胎的生长发育明显受到影响 (P <0 .0 5 ) ,胚胎畸形率和死亡率增高 (P <0 .0 5 )。当培养基pH为 5 .5时 ,培养胚胎死亡率达1 0 0 %。结论　全胚胎培养培养基pH条件改变 (过低或过高 )能够影响培养胚胎的生长发育。植入后全胚胎培养培养基最适pH值为 7.5～ 8.2。     

Characterization of Latent Transforming Growth Factor-β From Human Seminal Plasma

PROBLEM : Human seminal plasma is known to exhibit immunosuppressive activity. Transforming growth factor β (TGF-β) has been identified as an immunosuppressive factor in human seminal plasma. Biologically active TGF-β represents a family of 25-kDa homodimeric proteins linked with disulfide bonds. TGF-β associates with high molecular weight proteins noncovalently to form a type of latency that is biologically inactive. Quantitative distribution of active form of TGF-β versus inactive latent form of TGF-β, and mechanism of the TGF-β activation in human seminal plasma remain to be elucidated. PURPOSE : To characterize seminal plasma latent form of TGF-β, including its concentration, and the mechanism underlying the activation of TGF-β. METHOD : Gel filtrations on ACA-34 and Biogel P-60 were used to fractionate seminal plasma. TGF-β was measured by enzyme immunoassay using antibodies specific for TGF-β₁ and TGF-β₂, respectively. Radioreceptor assay with recombinant human [¹²⁵I]-TGF-β₁ was applied to qualitatively identify TGF-β₁. Kinetic experiments with various pH, temperature and time, along with protease inhibitors, were performed to delineate the activation mechanism of latent TGF-β. RESULTS : Human seminal plasma contained both TGF-β₁ and TGF-β₂, predominantly in latent form. The total concentration of TGF-β₁ averaged 238 ng/ml versus an average of 18 ng/ml for TGF-β₂. The in vitro activation or release of TGF-β₁, from latent TGF-β₁ was achieved only at acidic pH of <4.0, and was time and temperature dependent. At pH 3.7 and 37°C, a significant activation of latent TGF-β₁ was achieved after an incubation of only 15 min, reached the maximum at 120 min, and the activated TGF-β₁ remained relatively stable for at least 24 h. The activation was not inhibitable by a series of protease inhibitors examined, alone or in combination (e.g., phenylmethylsulfonyl fluoride, E-64, pepstatin, leupeptin, ethylenediamine tetraacetic acid). Competitive radioreceptor assay established the functional identity of TGF-β₁ in human seminal plasma with recombinant human TGF-β₁. CONCLUSION : Human seminal plasma TGF-β is biologically activated from high molecular weight latent TGF-β by acid pH. The acidic environment of female lower genital tract could represent an in vivo physiological condition for activation of seminal plasma TGF-β that may immunologically protect the integrity of sperm.