铜蒸气激光与光敏剂联合治疗鲜红斑痣的临床研究

铜蒸气激光与光敏剂ＰＳＤ—００７进行ＰＤＴ治疗鲜红斑痣３４０例，总有效率达９８．８％其中优良率７６．６％，无遗留任何疤痕。与单纯铜激光或氩激光光源相比，其优率Ｐ＜０．０１     

高效建立129S1/SvImJ 小鼠胚胎干细胞方法的探讨

选取超排后129S1/SvImJ品系小鼠的优质囊胚,使用辐照后冻存复苏的小鼠胚胎成纤维细胞作为饲养层,对比高浓度酶短时间消化法和低浓度酶长时间消化法,以0.25%胰酶-0.04%EDTA高浓度酶短时间消化法高效建立了4株小鼠胚胎干细胞系,建系率为36.31%.碱性磷酸酶,核型分析,体外分化和体内分化能力以及小鼠胚胎干细胞表面特异性分子标志0ct-4和Nanog的检测等表明,4个ES细胞系均为典型的小鼠胚胎干细胞系.所建立的ES细胞系为大规模培养ES细胞,进行后续的实验建立了理想的材料平台.     

不同激光参数照射下血管中血栓的演变

目前,激光是治疗葡萄酒色斑(Port Wine Stain,PWS)最有效的疗法。然而,由于选择性光热效应机理研究的欠缺,PWS的临床彻底清除率依然很低(<20%)。本文利用鼠脊视窗模型研究了不同激光参数照射下血管中光凝块和血栓的演变规律,以期为开发新的治疗策略提供依据。实验结果表明,Nd:YAG激光(1064 nm)照射后血管中只出现光凝块。长脉宽532nm激光照射后血管中首先形成光凝块,随着光凝块的流走,血栓产生并粘着血管壁。血栓面积随时间先增大后减小,存在时间长达4 h以上。短脉宽532 nm激光照射后,则形成非粘着血管壁血栓并随血流流走。由于形成完全堵塞血管的血栓是清除血管的前提,长脉宽532 nm激光联合抗血栓药物治疗PWS有望改善激光治疗PWS疗效。     

Improved conditions for periodate/Schiff's base‐based fluorescent staining of glycoproteins with dansylhydrazine in SDS‐PAGE

An improved periodate/Schiff's base based fluorescent stain with dansylhydrazine (DH) for glycoproteins in 1D and 2D SDS‐PAGE was described. Down to 4–8 ng of glycoproteins can be selectively detected within 2 h, which is approximately 16‐fold higher than that of original protocol, but similar to that of Pro‐Q Emerald 488 stain (Invitrogen, Carlsbad, USA). Furthermore, subsequent study of deglycosylation, glycoprotein affinity isolation, and LC‐MS/MS analysis were performed to confirm the specificity of the improved method. As a result, improved DH stain may provide a new choice for selective, economic, MS compatible, and convenient visualization of gel‐separated glycoproteins.     

Alternative visualization of SDS‐PAGE separated phosphoproteins by alizarin red S‐aluminum (III)‐appended complex

A novel fluorescence detection system using a chemosensor for phosphoprotein in gel electrophoretic analysis has been developed. The system employed the alizarin red S‐aluminum (III)‐appended complex as a fluorescent staining dye to perform the convenient and selective detection of phosphorylated proteins and total proteins in SDS‐PAGE, respectively. Therefore, a full and selective map of proteins can be achieved in the same process without resorting to other compatible detection methods. As low as 62.5 ng of α‐ (seven or eight phosphates) and β‐casein (five phosphates), 125 ng of ovalbumin (two phosphates), and κ‐casein (one phosphate) can be detected in approximately 135 min, with the linear responses of rigorous quantitation of changes over a 125–4000 ng range. As a result, alizarin red S‐aluminum (III) stain may provide a new choice for selective, economic, and convenient visualization of phosphoproteins.     

小剂量HpD配合可变脉宽532nm激光治疗鲜红斑痣的病理电镜研究

目的 :寻求治疗鲜红斑痣疗效佳、对正常皮肤损伤小、副反应小的方法。方法 :以不同剂量HpD配合不同剂量带同步冷却装置的可变脉宽 5 3 2nm激光照射鲜红斑痣动物模型来克享大公鸡鸡冠 ,在不同时间进行组织病理和超微结构的研究。结果 :治疗后即刻血管内皮细胞肿胀明显导致管腔闭塞 ,腔内见破坏的红细胞碎片 ,反应较单纯激光治疗组严重。结论 :小剂量HpD配合可变脉宽 5 3 2nm激光治疗鲜红斑痣可以提高疗效     

A statistical comparison of silver and SYPRO Ruby staining for proteomic analysis

Silver staining has been the method most commonly employed for high sensitivity staining of proteins following two-dimensional gel electrophoresis. Whilst this method offers detection in the nanogram range it does have major drawbacks including a lack of linearity, nonstoichiometric staining of proteins, a lack of compatibility with the microchemical preparation of proteins for identification by mass spectrometric techniques, and a highly subjective assessment of the staining endpoint. SYPRO Ruby is a relatively new, ruthenium complex-based stain which is reported to offer advantages over silver, particularly in overcoming the limitations cited above. We describe a series of experiments where several protein staining procedures commonly employed are compared. To enable optimization of the in situ digestion procedure, a statistical approach has been undertaken. The effects of a variety of staining, digestion, and analysis protocols on the downstream processing of a test radiolabeled protein were studied. The data confirms that as well as offering sensitivity similar to silver, SYPRO Ruby staining is reproducible, linear, and offers a higher level of compatibility with the identification of proteins by mass spectrometry.     

The monitoring of nucleotide diphosphate kinase activity by blue native polyacrylamide gel electrophoresis

Nucleoside diphosphate kinase (NDPK) has been shown to play a pivotal role in modulating a plethora of cellular processes. In this study, we report on a blue native (BN) PAGE technique which allows the facile assessment of NDPK activity and expression. The in-gel detection of NDPK relies on the precipitation of formazan at the site of immobilized enzyme activity. This is achieved by coupling the formation of ATP, as a consequence of gamma-phosphate transfer from NTP to ADP, to hexokinase (HK), glucose-6-phosphate dehydrogenase (G6PDH), oxidized nicotinamide adenine dinucleotide phosphate (NADP), phenazine methosulfate (PMS), and iodonitrotetrazolium chloride (INT). 2-D denaturing gel analysis confirmed that the activity bands corresponded to NDPK as indicated by subunit composition. Furthermore, the sensitivity and specificity of this readily accessible procedure was assessed by monitoring the in-gel activity of NDPK using different concentrations of GTP and CTP as well as deoxynucleoside triphosphates. This electrophoretic technique allows the quick and easy detection of NDPK, a housekeeping enzyme crucial to cell survival.     

Separation mixed semen of two individuals using magnetic beads coupled ABH blood group antibody

In sexual assault cases, one of the most common samples collected is a mixed semen stain, which is often found on the vagina, female underwear, or bed sheets. However, it is usually difficult to identify the perpetrator based on this sample alone. One technique that has been developed to address this issue is magnetic bead-based separation. This method involves using modified magnetic microspheres to capture and enrich specific target cells, in this case, sperm cells. In this study, we utilized magnetic beads coupled with ABH blood group antibody to isolate sperm cells from an individual of a single ABO blood type. Subsequently, polymerase chain reaction amplification and capillary electrophoresis were employed to perform the genotyping the short tandem repeat (STR) loci. This approach allows for the identification of different individuals in a mixed seminal stain sample from two individuals, by first separating sperm cells based on ABH antigen differences and subsequently utilizing autosomal STR typing on the enriched single blood group cells.     

A rapid and simple 8‐quinolinol‐based fluorescent stain of phosphoproteins in polyacrylamide gel after electrophoresis

In order to obtain an easy and rapid protocol to visualize phosphoproteins in SDS‐PAGE, a fluorescent detection method named 8‐Quinolinol (8‐Q) stain is described. 8‐Q can form ternary complexes in the gel matrix contributed by the affinity of aluminum ion (Al³⁺) to the phosphate groups on the proteins and the metal chelating property of 8‐Quinolinol, exhibiting strong fluorescence in ultraviolet light. It can visualize as little as 4～8 ng of α‐casein and β‐casein, 16～32 ng of ovalbumin and κ‐casein which is more sensitive than Stains‐All but less sensitive than Pro‐Q Diamond. The protocol of 8‐Q requires only 70 min in 0.75 mm mini‐size or 1.0 mm large‐size gels with five changes of solutions without destaining step; Pro‐Q takes at least 250 min with 11 changes of solutions. In addition, the new method was confirmed by the study of dephosphorylation and LC‐MS/MS, respectively. The approach to visualize phosphoprotein utilizing 8‐Q could be an alternative to simplify the analytical operations for phosphoproteomics research.