MgO–SBA-15 Supported Pd–Pb Catalysts for Oxidative Esterification of Methacrolein with Methanol to Methyl Methacrylate

Novel Mg O–SBA-15 supported catalysts were prepared for oxidative esterification of methacrolein(MAL) with methanol to methyl methacrylate(MMA). The Mg O–SBA-15 supports were synthesized with different magnesia loadings from different magnesium precursors and hydrochloric acid molar concentrations. The Mg O–SBA-15 supports and Pd–Pb/Mg O–SBA-15 catalysts were characterized by several analysis methods. The results revealed that the addition of Mg O improved the ordered structure of SBA-15 supports and provided surface alkalinity of SBA-15 supports. The average size of the Pd3 Pb particles on magnesia-modified Pd–Pb/Mg O–SBA-15 catalysts was smaller than that on the pure silica-based Pd–Pb/SBA-15 catalysts. The experiments on catalyst performance showed that the magnesia-modified Pd–Pb/Mg O–SBA-15 catalysts had higher activity than pure silica-based Pd–Pb/SBA-15 catalysts, showing the strong dependence of catalytic activity on the average size of active particles. The difference of activity between Pd–Pb/SBA-15 catalysts and Pd–Pb/Mg O–SBA-15 catalysts was due to the discrepant structural properties and surface alkalinity provided by Mg O, which led to the different Pd3 Pb particle sizes and then resulted in the different number of active sites. Besides magnesia loadings, other factors, such as hydrochloric acid molar concentration and magnesium precursors, had considerable influences on the catalytic activity.

预热处理温度对Ag-NH_(3)/SBA-15催化剂表面Ag物种形成及其催化性能的影响

采用浸渍法将有序介孔分子筛SBA-15浸渍于银氨溶液中制备催化剂前驱体,然后在不同预热处理温度下制备了Ag-NH_(3)/SBA-15系列催化剂样品,并考察了其催化草酸二甲酯(DMO)加氢制备乙醇酸甲酯(MG)的反应性能。结果表明:控制适当的预热处理温度(如623 K)有利于生成更多能与硅羟基形成Ag—O—Si键的Ag 2O颗粒,从而抑制Ag物种的团聚,提高表面Ag物种分散度,还有利于形成更多带部分正电荷的Ag^(δ+)活性位,使H_(2)分子更容易被活化,进而提高Ag-NH_(3)/SBA-15催化剂的活性;在温度为483 K、压力为2.0 MPa、H_(2)/DMO摩尔比为100、液时质量空速(MHSV)为1.4 h^(-1)的反应条件下,Ag-NH_(3)/SBA-15-623K催化剂作用下DMO的加氢转化率为97.9%、MG的选择性和收率分别为94.9%和92.9%。

METHYLATION PATTERN OF LRP15 GENE IN LEUKEMIA

Objective To investigate the methylation status of LRP15 gene in acute leukemia （AL） patients and its role in the tumorigenesis. Methods The methylation of LRP15 promoter and first exon of bone marrow mononuclear cells in 73 patients with AL, 10 with chronic leukemia （CL）, 9 with hematological benign diseases, and 20 healthy transplantation donors was analyzed by using methylation specific polymerase chain reaction. The methylation of LRP15 gene promoter and first exon in COS7, K562, and HL60 cell lines was also assayed. Resuits No LRP15 gene promoter methylation was detected in COS7 cell line. LRP15 gene promoter was methylated in K562 and HL60 cell lines. No deletion of LRP15 gene was detected in all samples. In nearly all French-American-British leukemia subtypes, we found that frequency of LRP15 methylation in adult patients with AL was 71.23% （ 52/73 ）. There was no detectable methylation in any of the 20 healthy donors and 8 chronic myeloid leukemia patients. The difference in frequency of LRP15 methylation between AL patients and healthy donors or CL patients （ 10.00%, 1/10） was significant （P 〈0.01 ）. Hypermethylation of LRP15 gene was found in 57.14% （16/28） of newly diagnosed AL patients, 83.33% of relapsed AL patients respectively, which was significantly different （ P 〈 0.05 ）. We also demonstrated LRP15 methylation in 55.56% （5/9） adults with benign hematological diseases. Conclusions LRP15 methylation changes are common abnormalities in leukemia. LRP15 is postulated to be a tumor suppressor gene.

DELETION AND 5'CPG ISLAND METHYLATION OF p15 GENE IN BRAIN GLIOMA

Objective: To investigate the abnormality of p15 gene in brain glioma and the correlation of it with occurrence or malignant progression of brain glioma. Methods: Deletion and 5'CPG island methylation of p15 gene were detected by the methods of PCR and PCR- based methylation in 56 cases of brain glioma. Results: Out of 43 cases of high grade glioma, 14 cases were found to have homozygous deletion of p15E1, while none of the 13 cases of low grade glioma was found to have deletion of p15E1 (P<0.05). Methylation of 5'CPG Island of p15 gene was found only in four cases of glioma. Conclusion: Abnormality of p15 gene may involved in the occurrence and malignant progression of brain glioma. Homozygous deletion of gene is the major mechanism of inactivation for p15 gene in brain glioma.

METHYLATION OF p16 AND p15 GENES IN MULTIPLE MYELOMA

Objective.To investigate the frequency of p16a nd p15gene methylation in multiple myeloma (MM),and its relationship with bone marrow ce ll apoptosis and clinical outcome.Methods.Twenty-two patients with MM were stu died to detect p16and p15gene methylation.Methyla-tion-specific polymerase chain rea ction(MSP)was used to detect gene methylation,and terminal trans-ferase-mediated dUTP nick end-labeling(TUNEL)was used to detect cell apoptosis.Results.p16and /or p15gene methylatoin was d etected in 10of 22patients(45.4%).There were 3pa-tients with p16gene methylation,9p atients with p15gene methylation,a nd 2patients with both genes methyla-tion.The incidence of methylation o f p15gene was higher than that of p16g ene(P<0.05).The patients with p16and /or p15gene methylation had a delayed cell apoptosis,poor respon se to chemotherapy,and a short over-all survival(OS).Conclusion.The methylation of p16and /or p15gen e plays a key role in MM apoptosis path ogenesis.The patients with both p16and p15gene me thylation had a poor prognosis.

SBA-15-[HSO_3-AMS]^+[HSO_4]^-催化合成松香甲酯

采用接枝的方法将功能化离子液体[HSO3-AMS]+[HSO4]-引入介孔分子筛SBA-15中,制备了SBA-15-[HSO3-AMS]+[HSO4]-,通过X射线衍射(XRD),红外(FI-IR)及吡啶吸附红外(Py-IR)对合成的材料进行了表征,结果表明接枝[HSO3-AMS]+[HSO4]-后的介孔分子筛与SBA-15相比,仍具有介孔结构且具有良好的长程有序性,具有大量的B酸和L酸中心。将制备的材料用于催化合成松香甲酯,结果表明SBA-15-[HSO3-AMS]+[HSO4]-具有较好的催化活性,较适宜的反应条件为:n(松香)∶n(甲醇)1∶30,反应温度200℃,反应时间5 h,催化剂用量为松香质量的6%,酯化率可达97.2%。且该催化剂具有较好的重复使用性。

介孔分子筛P-SBA-15催化合成油酸甲酯

对介孔分子筛SBA-15进行了磷酸改性,制备了P-SBA-15催化剂,用于油酸和甲醇的酯化反应。结果表明,P-SBA-15具有较好的催化活性和稳定性,是一种适用于大分子反应的固体酸催化剂。最佳酯化反应条件为:n(甲醇):n(油酸)=2:1,反应温度100℃,反应时间8 h,催化剂用量为原料质量的4．3％。

介孔分子筛Nb_2O_5/SBA-15催化合成油酸甲酯

以介孔分子筛SBA-15为载体,采用浸渍法合成了Nb2O5/SBA-15催化剂。通过XRD、BET等测试手段对样品进行了分析。结果表明,负载Nb2O5的SBA-15分子筛具有高度有序的二维六方介孔结构,并且具有较大的比表面积、孔容和孔径。Nb2O5/SBA-15分子筛催化剂的酯化反应最佳反应条件为:醇酸物质的量比为2∶1,反应温度160℃,反应时间4 h,催化剂用量为原料总质量的9.10%。Nb2O5/SBA-15催化剂具有较好的稳定使用性,是一种合成油酸甲酯的理想固体酸催化剂。

消旋（15R）－15甲基PGE_2甲酯（PG_6E）对大鼠实验性胃溃疡的保护作

用实验性胃溃疡模型研究了ＰＧ＿６Ｅ的抗溃疡作用，结果表明ＰＧ＿６Ｅ有抗胃酸分泌作用，而对胃肠运动无明显影响；ＰＧ＿６Ｅ在剂量为１０一８０μｇ·ｋｇ－１时，对无水乙醇型、盐酸型、消炎痛型、慢性醋酸型和幽门结扎型胃溃疡有明显保护作用，并能显著减少幽门结扎大鼠的胃液体积、胃酸分泌、胃蛋白酶活性和ＤＮＡ含量。小鼠ｐｏＰＧ＿６Ｅ３０～６０μｇ·ｋｇ－１，３ｄ后粘膜氨基己糖含量显著增加。研究结果提示ＰＧ＿６Ｅ能抑制对胃粘膜的攻击性因素，增加保护性因素的作用。

介孔分子筛K_2O/SBA-15催化酯化反应的研究

以介孔分子筛SBA-15为载体,负载KNO3后经过煅烧,制得K2O/SBA-15固体碱催化剂。通过XRD和BET对样品进行了测试分析,并对K2O/SBA-15催化合成油酸甲酯的酯化反应进行了研究。试验结果表明:当K2O负载量为2%,n(醇)∶n(酸)2∶1,反应温度180℃,反应时间4 h,催化剂用量为原料质量的5.0%时,酯化率最大达到83.61%,并且K2O/SBA-15催化剂重复使用多次仍具有较好的催化效果。

WO_3/SBA-15催化剂的制备及其氧化脱硫性能

以介孔SBA-15分子筛为载体,采用两种不同钨源(H_2WO_4和H_2C_2O_4、H_2WO_4和H_2O_2)通过浸渍法制备了WO_3/SBA-15催化剂;采用X射线衍射和傅里叶变换红外光谱法对介孔SBA-15分子筛和WO_3/SBA-15催化剂进行了表征;以硫含量为500μg/g的模拟汽油为原料进行氧化脱硫反应,反应后油相用1-甲基-2-吡咯烷酮萃取,考察了萃取剂用量、催化剂用量、氧化反应温度和反应时间对脱硫率的影响。表征结果显示,WO_3/SBA-15催化剂有规则的二维六方介孔结构,WO_3在载体上高度分散。实验结果表明,以H_2WO_4和H_2C_2O_4为钨源制备的WO_3/SBA-15催化剂的脱硫效果较好,在反应温度320 K、反应时间120 min、模拟汽油60 mL、催化剂用量0 12 g、双氧水0.57 mL、萃取剂与模拟汽油体积比0.50、萃取时间5 min的条件下,脱硫率可达94.05%。

联合应用dI-15-甲基PGF_(2α)与RU486抗早孕的临床研究

本文报道80例早孕≤49天,用不同剂量dl-15-甲基PGF_(2α)(以下简称PG)与不同剂量RU486配伍,分成三组,进行抗早孕比较,结果三组成功率达100%,完全流产率94.87%。三组完全流产率无显著差异。组ⅢRU486 25mg,每日2次,2天总量100mg,第三天加PG 0.5mg 肌注,完全流产率95%,大大减少PG 用量,明显减轻了副反应,为三组首选抗早孕配伍。为目前国内外报道抗早孕的RU486最小剂量。

双炔失碳酯或丙睾配伍dl-15甲基PGF_(2α)抗早孕的临床比较

本文报告65例双炔失碳酯配伍d1-15甲基PGF_(2α)(以下简称PG)抗早孕结果并与33例丙睾配伍PG抗早孕结果进行比较。结果显示,双炔失碳酯组完全流产59例,占90%;不全流产3例,占5%;失败3例,占5%;总有效率95%。丙睾组完全流产27例,占82%;不全流产6例,占18%;总有效率100%。两组总有效率无显著差异;完全流产率无显著差异;但不全流产率有明显差异(P<0.05)。药流后点滴出血天数,双炔失碳酯组平均为8.1±5.0天;丙睾组平均为18.9±19.1天;两组有明显差别(P<0.05)。双炔失碳酯经阴道给药后无一例发生心、肝、肾功能变化。

Ce改性SBA-15分子筛催化合成棕榈酸甲酯

用浸渍法对SBA-15分子筛进行Ce改性，制备了Ce（SO4）2／SBA-15催化剂，采用X射线衍射、红外光谱、N2吸附-脱附、热重-差热分析方法对试样进行了表征。表征结果显示，Ce已进入SBA-15分子筛中，制得的Ce（SO4）2／SBA-15催化剂保持高度有序的介孔二维六角结构。用Hammett指示剂法测得ce（SO4）2／SBA-15催化剂的表面酸强度为0．99—1．80，酸量为0．2344mmol／g。采用Ce（So4）2／SBA-15催化剂催化甲醇和棕榈酸酯化合成棕榈酸甲酯，优化的合成条件为：n（棕榈酸）：n（甲醇）=1：15，催化剂用量为棕榈酸质量的5．0％，反应时间8h。在此条件下，酯化率大于92％。

SO_4^(2-)/Al_2O_3-ZrO_2/SBA-15固体酸催化合成棕榈酸甲酯

将Al(NO3)3.9H2O,Zr(NO3)4.5H2O与活化后的主体材料SBA-15分子筛通过尿素水解的方法,制备了改性SBA-15分子筛,进一步用硫酸浸渍处理改性分子筛以增强分子筛表面的酸活性中心。并采用红外光谱、扫描电镜、透射电镜等分析方法对试样进行了表征,结果表明,制得的催化剂SO24-/Al2O3-ZrO2/SBA-15仍然保持高度有序的介孔一维六角结构。并将其催化剂用于棕榈酸与甲醇的酯化反应中,采用正交实验确定较佳的工艺条件为:催化剂用量为1.2 g,n(棕榈酸)∶n(甲醇)=1∶12,反应时间为9 h,此条件下棕榈酸甲酯的反应收率可以达到82.3%,实验表明所合成的固体酸催化剂具有良好的催化性能。

(±)和(+)15-甲基PGF_(2α)甲酯的抗早孕作用

15－甲基PGF2α甲酯（PG05）对小鼠有明显的抗早孕作用。（＋）PGOS为有活性的立体异构体，其抗早孕和致腹泻作用均比（±）PGOS强，治疗指数与（±）PG05基本一致。大鼠于妊娠第7、8、9天，皮下注射（±）PG050.5mg／kg有明显的抗早孕作用；同样剂量的PGOS对去卵巢后，靠外源性孕酮和雌酮维持妊娠的大鼠无抗早孕作用。PGOS20μg／ml既可抑制hCG刺激黄体细胞分泌cAMP，又能桔抗SBr－cAMP刺激黄体细胞分泌孕酮，PG05可能在2个或2个以上环节上抑制大鼠卵巢黄体功能。

Amberlyst-15催化丁酮氧化制备过氧化甲乙酮

作为一种新型绿色催化剂,离子交换树脂能够代替某些有机反应中的传统催化剂。本文以离子交换树脂Amberlyst-15为催化剂,由30%的双氧水、丁酮和稀释剂邻苯二甲酸二丁酯合成过氧化甲乙酮。在双氧水与丁酮的摩尔比为1.0,离子交换树脂与丁酮的质量比为0.06,反应温度为27℃,反应时间55 min的条件下,过氧化甲乙酮的产率接近86%,活性氧含量为12.9%。Amberlyst-15在循环使用8次后,依然保持良好的稳定性。研究表明:Amberlyst-15用于过氧化甲乙酮的制备具有催化活性高、可重复使用、清洁无腐蚀等优点,为工业环保生产有机过氧化物提供了新途径。

微波辅助ZrO_2-SO_4^(2-)/SBA-15催化合成棕榈酸甲酯

以三嵌段醚共聚物P123作为模板剂、正硅酸乙酯为硅源,合成介孔分子筛SBA-15。以SBA-15为载体,利用尿素水解法制备ZrO2-SO24-改性的固体酸催化剂,对其进行表征。实验结果表明,合成的固体酸催化剂具有典型的介孔结构特征。将催化剂应用于微波法催化合成棕榈酸甲酯,考察反应时间、反应温度、辐射功率、酸醇物质的量比和催化剂用量对酯化率的影响,结果表明,在n(十六酸)∶n(甲醇)=1∶15、SZ/SBA-15催化剂用量0.8 g、反应时间20 min、反应温度40℃和微波辐射功率400 W条件下,酯化率可达87.70%,微波反应时间较传统合成方法大大缩短。

Fe-壳聚糖/SBA-15催化潜手性酮不对称氢转移反应

以SBA-15介孔分子筛为载体制备了Fe(Ⅲ)-壳聚糖(CS)络合物为活性组分的多相手性催化剂(Fe-CS/SBA-15)。以异丙醇作氢源,在常压下Fe-CS/SBA-15催化剂用于苯乙酮和4-甲基-2-戊酮不对称氢转移反应,考察了Fe-CS/SBA-15催化剂中Fe含量、反应温度、反应时间及助催化剂KOH浓度对底物转化率和产物对映选择性的影响规律。实验结果表明,Fe-CS/SBA-15催化剂中适宜的Fe质量分数为2.2%;对于苯乙酮和4-甲基-2-戊酮不对称氢转移反应,适宜的反应条件为:KOH浓度0.03m ol/L,反应温度70℃,反应时间分别为4,8h。在此条件下,苯乙酮的转化率为27.7%,产物R-1-苯乙醇的对映体过量(ee)值为87.4%(4h);4-甲基-2-戊酮的转化率为25.5%,产物R-4-甲基-2-戊醇的ee值为50.2%(8h)。

痰标本p16基因启动子区甲基化联合血清细胞角蛋白19片段和癌抗原15-3对非小细胞肺癌的诊断价值

目的评价痰液标本中p16基因启动子区甲基化联合血清中细胞角蛋白19片段(cytokeratin 19 fragment,CYFRA 21-1)和癌抗原15-3(CA15-3)的检测对非小细胞肺癌(NSCLC)的诊断价值。方法用巢式甲基化特异性聚合酶链反应(MSP)检测100例NSCLC患者痰液p16基因启动子区甲基化联合化学发光法检测患者血清中CYFRA21-1和CA15-3的水平,评价3种肿瘤标志物联合检测对NSCLC的诊断价值。结果NSCLC患者痰液中p16基因启动子区甲基化阳性率为61.0%;NSCLC患者血清中CYFRA21-1和CA15-3的实验敏感度分别为58.0%和38.0%;联合检测可明显提高NSCLC的检出率,敏感度79.0%,明显高于各种肿瘤标志物单项检测。结论痰液标本中p16基因启动子区甲基化联合血清中CYFRA21-1和CA15-3的检测可明显提高NSCLC的检出率,为早期诊断NSCLC提供了依据。