Synthesis,molecular docking,and biological activity of 2-vinyl chromones: Toward selective butyrylcholinesterase inhibitors for potential Alzheimer's disease therapeutics

We investigated the biological activity of a series of substituted chromeno[3,2-c]pyridines, including compounds previously synthesized by our group and novel compounds whose syntheses are reported here. Tandem transformation of their tetrahydropyridine ring under the action of activated alkynes yielding 2-vinylsubstituted chromones was used to prepare nitrogen-containing derivatives of a biologically active chromone system. The inhibitory activity of these chromone derivatives against acetylcholinesterase (AChE), butyrylcholinesterase (BChE) and carboxylesterase (CaE) was investigated using the methods of enzyme kinetics and molecular docking. Antioxidant (antiradical) activity of the compounds was assessed in the ABTS assay. The results demonstrated that a subset of the studied chromone derivatives selectively inhibit BChE but do not exhibit antiradical activity. In addition, the results of molecular docking effectively explained the observed features in the efficacy, selectivity, and mechanism of BChE inhibition by the chromone derivatives.     

风湿性心脏病瓣膜置换术患者围术期血浆脑钠肽水平的表达及临床意义

目的:探讨风湿性心脏病瓣膜置换术患者围手术期血浆脑钠肽(BNP)水平及其临床意义。方法:选取2015年1月至2016年12月在我院接受心脏瓣膜置换术的风湿性心脏病患者98例为研究对象,分别于术前、术后12 h、24 h、48 h、术后1周进行血浆BNP、磷酸肌酸同工酶(CK-MB)、高敏C反应蛋白(hs-CRP)水平检测,观察纽约心脏病协会(NYHA)不同心功能分级、不同时间点患者血浆BNP、CK-MB、hs-CRP水平变化,同时观察并比较术后发生严重心律失常与否的患者在不同时间点血浆BNP、CK-MB、hs-CRP水平变化。结果:随NYHA心功能分级升高,患者血浆BNP、CK-MB、hs-CRP水平升高,不同NYHA心功能分级患者血浆BNP、hs-CRP水平比较差异有统计学意义(P0.05),CK-MB水平比较差异无统计学意义(P0.05);不同NYHA心功能分级患者血浆BNP、hs-CRP两两比较差异有统计学意义(P0.05),CK-MB两两比较差异无统计学意义(P0.05)。患者术后12 h、24 h、48 h血浆BNP、hs-CRP水平均显著高于术前,术后24 h、48 h血浆CK-MB水平均显著高于术前,而术后1周血浆BNP、CK-MB、hs-CRP显著低于术前(P0.05)。术后发生严重心律失常(严重心律失常组)患者16例,未发生严重心律失常(无严重心律失常组)患者82例,两组患者术后12 h、24 h、48 h血浆BNP、CK-MB、hs-CRP水平均显著高于术前(P0.05);两组患者术后1周BNP与术前比较差异无统计学意义(P0.05),而CK-MB、hs-CRP水平均显著低于术前(P0.05),但严重心律失常组术后12 h、24h、48 h、1周血浆BNP、CK-MB、hs-CRP水平均显著高于无严重心律失常组(P0.05)。结论:风湿性心脏病瓣膜置换术患者术前血浆BNP可以反映患者心功能情况,术后患者血浆BNP、CK-MB、hs-CRP异常升高,发生严重心律失常患者升高更为明显。     

一例母及其亲子DNA指纹与血清蛋白、酯酶遗传的研究

采用ＤＮＡ指纹分析和聚丙烯酰胺凝胶电泳法,对一例与公驴交配生育了后代的母后代进行了亲缘鉴定和血清蛋白、酯酶遗传的分析。结果可以认定其亲子关系并证实母骡生育的事实。虽然本例母的后代在Ｐｒ、Ａｌ、Ｐａ和Ｈｂ、Ｅｓ等基因座位上的基因表达倾向于驴,但其外貌仍明显地带有种间杂种的特征。因此,尚不能简单地认为其已“回归”为纯种的驴。     

小牛碱性磷酸酶同工酶的一些特性

我们用正丁醇抽提,经ＳｅｐｈａｄｅｘＧ－１００凝胶过滤和ＤＥＡＥ－纤维素柱层析两步纯化,得到了比活性增大４０倍和ＰＡＧＥ纯的牛ＡＫＰ同工酶。对各ＡＫＰ同工酶分别进行酶活性、电泳迁移率（Ｒｆ值）、热抑制、尿素抑制、组织特异性抑制实验,以鉴别每种同工酶的特性。实验结果表明：①各同工酶Ｒｆ值,肝同工酶＞骨同工酶＞小肠同工酶;②经５６℃加热１０ｍｉｎ,只有骨同工酶完全失活,而肠同工酶对热是稳定的;③尿素强烈地抑制骨同工酶活性;肠同工酶对尿素是稳定的;④组织特异性抑制剂苯丙氨酸强烈抑制肠ＡＫＰ活性。     

Two 17beta-hydroxysteroid dehydrogenases (17HSDs) of estradiol biosynthesis: 17HSD type 1 and type 7.

Two 17β-hydroxysteroid dehydrogenases (17HSDs), type 1 and type 7, are enzymes of estradiol biosynthesis, in addition to which rodent type 1 enzymes are also able to catalyze androgens. Both of the 17HSDs are abundantly expressed in ovaries, the type 1 enzyme in granulosa cells and type 7 in luteinized cells. The expression of 17HSD7, which has also been described as a prolactin receptor-associated protein (PRAP), is particularly up-regulated in corpus luteum during the second half of rodent pregnancy. A moderate or slight signal for mouse 17HSD7/PRAP mRNA has also been demonstrated in samples of placenta and mammary gland, for example. Human, but not rodent, 17HSD1 is expressed in placenta, breast epithelium and endometrium in addition to ovaries. A cell-specific enhancer, silencer and promoter in the hHSD17B1 gene participate in the regulation of type 1 enzyme expression. The enhancer consists of several subunits, including a retinoic acid response element, the silencer has a binding motif for GATA factors, and the proximal promoter contains adjacent and competing AP-2 and Sp binding sites.     

盐碱胁迫下星星草种子萌发过程中有机物,呼吸作用及其几种酶活性的变化

对NaCO3胁迫下星星草种子萌发过程中淀粉酶活性、淀粉酶同工酶、可溶性糖含量、呼吸作用的变化进行了研究。结果表明无盐胁迫下,种于萌发过程中淀粉酶活性、可溶性糖含量、呼吸强度与对照相比均下降,并与Na2CO3胁迫浓度的负相关关系极其显著。Na2CO3胁迫下,水解酶活性降低、储藏物质不能动员、呼吸代谢受抑制是盐胁迫下星星草种子萌发受抑制的原因之一。     

Studies on the Esterase Isozymes in the New Lines of Progeny of the F1 Hybrid Rice

The new lines Nanhua 5, Nanhua 11, Shanyou 39, and Shanyou 59, are high-yield lines derived from the F1 hybrid rice, Nanyou 2 and Shanyou 2 by means of tissue culture and selec- tion. Five isozymes, esterase, peroxidase, ATP-ase, malate dehydrogenase and glulamate dehydrogenase from the new lines, the F1 hybrid rices and their parents, were analyzed by starch and polyacrylamid gel electrophoresis. There are no difference in zymogrames of ATPase, malate dehydrogenase, glulamate dehydrogenase, between the F1 hybrid and its parents. But the F1 hybrid rice contains complemental bands of anodal esterase EA2, EA3 and cathodal esterase EC1, EC2, EC3, EC4, The esterase zymogram of seeds of Nanhua 5, Nanhua 11 and Shanyou 39, Shanyou 59 could be observed in the progeny of the F2 hybrid rice. The results indicated that the new lines would be possibly derived from the progeny of the F1 hybrid by means of tissue culture and selection.     

Evidence for a constitutive cytoplasmic cutinase in ungerminated conidia of Botrytis cinerea Pers.: Fr.

Cytoplasmic soluble proteins from ungerminated conidia of Botrytis cinerea exhibited cutinase activity, while cell wall binding proteins lacked this activity. Cutinase activity in proteins extracted from cell walls and cytoplasm of ungerminated conidia of Botrytis cinerea was determined using p-nitrophenyl butyrate (PNB) and TLC analysis of products derived from hydrolysis of [³H]cutin. Treatment of conidia with indoxyl acetate, a substrate indicative of non-specific esterase and cutinase activity, also gave a positive reaction in the cytoplasm of ungerminated conidia. The possible role of a putative constitutive cutinase in the cytoplasm of conidia in the early stages of infection of plants by B. cinerea is discussed.     

南海深海微生物酯酶EST12-7在制备(R)-2-氯丙酸乙酯中的应用研究

利用来源南海深海的微生物酯酶EST12-7不对称水解反应拆分制备（R）-2-氯丙酸乙酯。并探寻了温度、pH、底物浓度、有机溶剂和反应时间等因素对酯酶EST12-7催化制备（R）-2-氯丙酸乙酯的影响。结果表明,深海微生物酯酶EST12-7催化制备（R）-2-氯丙酸乙酯的最佳反应条件为：13.8 μg/ml酯酶EST12-7,50 mmol/L（±）-2-氯丙酸乙酯,2%正癸醇,pH8.5,30℃,0.05mol/L Tris-HCl,反应60 min。在最佳反应条件下,（±）-2-氯丙酸乙酯的转化率可达49%,所制备的（R）-2-氯丙酸乙酯的光学纯度为98%。通过对酯酶EST12-7拆分制备（R）-2-氯丙酸甲酯和（R）-2-氯丙酸乙酯进行比较,2-氯丙酸酯中的链长对酯酶EST12-7拆分反应有极大的影响。     

Extracellular secretion of Pseudoalteromonas sp. cold-adapted esterase in Escherichia coli in the presence of Pseudoalteromonas sp. components of ABC transport system

Recently we described identification and characterization of GDSL esterase EstA from psychrotrophic bacterium Pseudoalteromonas sp. 643A. Attempts to obtain heterologous overexpression of this enzyme in Escherichia coli system were not satisfactory. The EstA protein was expressed as inclusion bodies, most of that were inactive after purification step, and the recovery of esterolytic activity was very low after refolding. Based on the sequence analysis we found that the esterase EstA gene is clustered with three genes encoding components of ABC transport system. These genes, designated abc1, abc2, and abc3 encode an ATP-binding protein (ABC1) and two permease proteins (ABC2 and ABC3). In present study, to obtain larger amounts of the active cold-adapted EstA esterase from Pseudoalteromonas sp. 643A, we designed a two-plasmid E. coli expression system where the gene encoding EstA enzyme was cloned into pET30b(+) expression vector and three genes encoding components of ABC transport system were cloned into pACYC-pBAD vector. It was shown that the created expression system was useful for extracellular production of active EstA enzyme which was purified from the culture medium. In the presence of all the three transporter proteins the secretion of EstA was at the highest level. When one or two of these components were missing, EstA secretion was also possible, but not so effective. It indicates that ABC2 and ABC3 proteins of Pseudoalteromonas sp. 643A could be replaced with their homologous proteins of E. coli.