Isolation and characterization of human monoclonal antibodies specific to MMP-1A, MMP-2 and MMP-3

Matrix metalloproteinases (MMPs), a group of more than 20 zinc-containing endopeptidases, are up-regulated in many diseases, but the use of MMP inhibitors for therapeutic purposes has often been disappointing, possibly for the limited specificity of the drugs used in clinical trials. In principle, individual MMPs could be specifically drugged by monoclonal antibodies, either by inhibition of their catalytic activity or by antibody-based pharmacodelivery strategies. In this article we describe the isolation and affinity maturation of recombinant antibodies (SP1, SP2, SP3) specific to the murine catalytic domains of MMP-1A, MMP-2 and MMP-3. These novel reagents allowed a systematic comparative immunofluorescence analysis of the expression patterns of their cognate antigens in a variety of healthy, cancerous and arthritic murine tissues. While all three MMPs were strongly expressed in tumor and arthritis specimens, MMP-1A was completely undetectable in the normal tissues tested, while MMP-2 and MMP-3 exhibited a weak expression in certain normal tissues (e.g., liver). The new antibodies may serve as building blocks for the development of antibody-based therapy strategies in mouse models of pathology.     

Isolation of Myrosinase Producing Microorganism

Screening tests were undertaken to obtain microorganisms which produce myrosinase. One strain of microorganism indicated a strong capasity for producing myrosinase. The morphological and physiological characteristics of this strain were studied. The organism was identified as Enterobacter cloacae, no. 506.

Enzyme production was induced by the addition of 0.01% sinigrin and 6% mustard extract*² to the culture medium. The highest production was obtained after 36~40 hr cultivation when the strain was cultivated at 28°C in a medium containing 0.01% sinigrin, 6% Mustard ext., 0.1% KH₂PO₄, 0.1% NH₄Cl, 0.1% NaCl and 0.1% MgSO₄·7aq, (pH 7.0).     

一株表面活性剂产生菌的筛选及其特性研究

从氧化沟含油污水中分离得到1株能产生物表面活性剂菌株S6(Pseudomonas sp.),经生理生化实验和16SrDNA序列分析鉴定,S6为铜绿假单胞菌。红外光谱分析得知S6在代谢过程中能够产生糖脂类表面活性物质。其临界胶束浓度(CMC)为50mg/L,可将水的表面张力由72mN/m降到33.9mN/m。发酵液的表面张力和排油直径的测定结果显示发酵液在不同的盐度、pH和溶解氧量条件下,具有较稳定的表面活性。通过正交实验确定了优化培养基条件为葡萄糖10g、尿素5g、磷酸二氢钾1g、微量元素液2mL、pH8.0、水1000mL;S6在优化培养基中合成生物表面活性剂的产量为0.173g/L。     

Isolation and Identification of a Pyrogallol Oxidase Producing Microorganism and the Enzyme Production

A carbazole-using bacterium was isolated from oil polluted soil and identified as Flavobacterium sp. OCM-1 from its taxonomical characteristics. Its optimal culture conditions were identified. The growth and carbazole-degradation were found in the ranges of 20–30°C and pH 6–8. We found microbial production of indole-3-acetic acid from carbazole by strain OCM-1. Indole-3-acetic acid was identified as a metabolite of carbazole using thin-layer chromatography, mass and ¹H-NMR-spectra. 1.5 mg of indole-3-acetic acid was formed from 250 mg of carbazole.     

小鼠外胎盘锥次级滋养层巨细胞的分离、培养与鉴定

目的：建立小鼠外胎盘锥次级滋养层巨细胞的分离、培养方法.方法：在小鼠妊娠第8 d,通过机械分离和组织块翻转干涸法分离、培养小鼠外胎盘锥次级滋养层巨细胞;免疫细胞化学鉴定细胞来源与纯度;酶谱方法检测其所分泌基质金属蛋白酶2和9（matrix metalloproteinase-2,9,MMP-2,9）结果：利用机械分离法分离外胎盘锥可生长于Matrigel包被的培养板上,并生长出次级滋养层巨细胞,表达特异性标志物Cytokeratin;体外培养24 h、48 h后,外胎盘锥滋养层巨细胞的粘附率分别为（83.3±9.1）%和（92.4±7.3）%;扩展率分别为（45.5±5.3）%和（56.4±6.8）%;及其所分泌的MMP-2,9的24 h光密度值分别为（87±4.7）和（351.5±25.2）;48 h分别为（186±40.2）和（556.5±61.5）.结论：采用机械分离和组织块翻转干涸法,可简单、快捷地获得高纯度小鼠外胎盘锥次级滋养层巨细胞.     

Isolation and Identification of ATP: Nucleotide Pyrophospho-transferase-producing Microorganism

ATP: nucleotide pyrophosphotransferase-producing microorganism was isolated from soil in Osaka prefecture. The morphological and physiological characteristics of this microorganism were studied. This strain was identified and named Streptomyces adephospholyticus nov. sp.

When this strain was aerobically cultured in a fermentor at 30°C in a medium containing 2% glycerol, 4% polypepton, 0.1 % KH₂PO₄, 0.04% MgSO₄ · 7H₂O, 2 ppm FeSO₄ · 7H₂O and 2 ppm MnSO₄ · 6Н₂О at pH 7.0, ATP; nucleotide pyrophosphotransferase was produced in the culture filtrate. The highest activity was obtained after 30 to 40 hr cultivation. The maximum enzyme production was 3000 to 4000 unit per liter.     

Isolation of Metallo-proteinase Inhibitor (FMPI) Producing Microorganism

A screening test was carried out for the purpose of isolating a microorganism which produced a specific proteinase inhibitor for mold metallo-proteinase. A potent strain identified as Streptomyces rishiriensis was isolated, and this inhibitor was named fungal metallo-proteinase inhibitor (FMPI). The strain was aerobically cultured at 25°C for 26–30 hr in shaking flasks with a medium consisting of 1 % meat extract, 1 % polypepton and 0.3% NaCl (about 100 mg/liter). FMPI showed execellent inhibitory activity against the metallo-proteinase of Aspergillus oryzae, and moderate activity against other microbials. FMPI has a low molecular weight and is stable only at alkaline region (pH > 11).     

Isolation and Identification of a Microorganism Producing Bilirubin Oxidase

For the purposes of decoloring raw sewage and use as an analytical tool in clinical fields, we tried to obtain microorganisms producing an enzyme which is reactive to bilirubin. One strain of microorganism (MT-1) showed strong ability to produce the enzyme.

The morphological and physiological characteristics of strain MT-1 were studied. This strain was found to belong to Myrothecium verrucaria.

For the production of the enzyme, this strain was aerobically cultured at 25°C in a jar fermentor which contained potato-glucose medium. The highest activity was obtained after 62-hr cultivation.

This enzyme was also produced by other strains belonging to Myrothecium.     

Isolation and immunological characterization of an iron-regulated,transformation-sensitive cell surface protein of normal rat kidney cells

We have analyzed the surface proteins of cultured normal rat kidney (NRK) cells and virus-transfromed NRK cells subjected to iron deprivation. Such a treatment specifically induces two transformation-sensitive plasma membrane-associated glycoproteins with a subunit molecular wegiht of 160,000 (160 K) and 130,000 (130 K) daltons in NRK cells. In these cells the 160 K glycoprotein is readily available to lactoperoxidase-mediated iodination, and the 130 K is apparently inaccessible to iodination. Major differences were revealed when iodinated membrane proteins of normal and virus-transformed cells subjected to iron deprivation were compared. In Kirsten sarcoma virus-transformed NRK cells the 160 K glycoprotein was weakly labeled. In two clones of simian virus 40-transformed NRK cells the 160 K glycoprotein was weakly labeled or not at all. The 130 K glycoprotein was inaccessible to iodination in all the virus-transformed cell lines. The 160 K and 130 K glycoproteins were isolated form plasma membranes of NRK cells using preparative SDS gel electrophoresis. Antibodies generated against these glycoproteins stained the external surfaces of NRK cells and induced antigen redistribution. Evidence presented suggests that 160 K and 130 K are plasma membrane-associated procollagen molecules. A possible interaction of these proteins with transferrin is also described. The data suggest that these proteins may have an important role in the sequence of events leading to transformation.     

曾候乙墓穴木椁微生物的分离与鉴定

从曾侯乙墓中椁室、东椁室、西椁室和北椁室分别取样,经平板划线培养,分离,纯化共获得典型的菌株16株。将16株分别涂片镜检,生理生化分析鉴定,结果证明芽孢杆菌属11株,其中苏云金变种1株,地衣芽孢杆菌1株,巨大芽孢杆菌1株,球形芽孢杆菌5株,蜡状芽孢杆菌2株,多粘芽孢杆菌1株。其余菌株微杆菌属4株,黄色杆菌属黄杆菌1株。     

红霉素对慢性阻塞性肺疾病大鼠ICAM-1、MMP-9的表达影响

目的:观察慢性阻塞性肺疾病(COPD)大鼠肺组织中ICAM-1及MMP-9的表达及红霉素的干预作用。方法:复制COPD大鼠模型,并用红霉素干预,收集支气管肺泡灌洗液行细胞学计数和分类检查;采用HE染色观察病理形态变化;免疫组化法检测大鼠支气管肺组织ICAM-1、MMP-9的表达。结果:与模型组比较,干预组支气管肺组织中ICAM-1、MMP-9表达显著降低;模型组中ICAM-1、MMP-9的表达与BALF中白细胞总数及中性粒细胞数成正相关;ICAM-1与MMP-9的表达成正相关。结论:COPD大鼠肺组织中的ICAM-1、MMP-9表达明显升高,可能与COPD的发病机制有关;红霉素可降低ICAM-1、MMP-9的表达,可能是红霉素在COPD中抗炎症反应的作用机制之一。     

The Composition of Saccharogenic Amylase from Rhizopus javanicus and the Isolation of Glycopeptides

Saccharogenic amylase from Rhizopus javanicus sp. 3–46 was known to be a glycoprotein which contained 27 residues of mannose and 4 residues of N-acetylglucosamine per mole of the saccharogenic amylase. Attempts have been made to obtain glycopeptides from the saccharogenic amylase. Three glycopeptides, GP-I-a, GP-I-b and GP-II, were separated from a Pronase digest of heat-denatured saccharogenic amylase by gel filtration on Sephadex G-50 and chromatography on DEAE-Sephadex A-25. GP-I-a contained asparagine, glycine, mannose and N-acetylglucosamine in a molar ratio of 1: 1: 6: 2. GP-I-b contained asparagine, threonine, mannose and N-acetylglucosamine in a molar ratio of 1: 1: 9:2. GP-II consisted of threonine, serine, proline, alanine and mannose in a molar ratio of 6: 2: 2: 2: 12.     

MMP-9、TIMP-1及细菌L型在卵巢乳头状癌中的表达及意义

目的探讨MMP-9、TIMP-1及细菌L型在卵巢上皮性肿瘤中的表达及临床意义。方法采用原位杂交和免疫组化及革兰染色方法检测97例卵巢乳头状癌及23例卵巢乳头状瘤组织中MMP-9、TIMP-1的表达及细菌L型检出率,并用2χ检验进行统计学处理。结果卵巢乳头状癌中MMP-9及TIMP-1的表达率均明显高于良性肿瘤(P<0.005)。MMP-9在卵巢乳头状癌中临床分期Ⅲ、Ⅳ期中的表达率明显高于Ⅰ、Ⅱ期(P<0.005~P<0.01),随着病理分级增高而显著增加(P<0.005~P<0.05),腹腔淋巴结有转移和有腹水者均高于无腹腔淋巴结转移和无腹水者(P<0.005~P<0.05)。而TIMP-1阳性表达与MMP-9阳性表达相反,呈负相关。细菌L型检出阳性率与病理分级及临床分期差异有显著性,腹腔淋巴结有转移比无转移者、有腹水比无腹水者差异有显著性(P<0.005)。结论MMP-9、TIMP-1基因及蛋白在卵巢肿瘤中有不同程度的异常表达,两者均可作为判断卵巢肿瘤生物学行为及患者预后参考指标。L型感染极有可能成为诱发肿瘤因素之一,它与MMP-9、TIMP-1可能有协同致瘤及恶性肿瘤侵袭和转移作用。研究细菌L型感染与肿瘤的关系,具有重要的临床应用价值。     

Rice bran supplement prevents UVB-induced skin photoaging in vivo

Although rice bran consumption is reportedly has numerous beneficial effects on human health, the relationship between rice bran and the prevention of photoaging has not been investigated in detail. We sought to investigate whether consumption of rice bran supplement (RBS) can elicit preventive effects against UVB-induced photoaging in vivo. Dorsal skin sections of hairless mice were exposed to UVB over 16 weeks. RBS consumption suppressed UVB-induced wrinkle formation and inhibited the loss of water content and epidermal thickening in the mouse skin. Western blot and immunohistochemical analyses revealed that repeated exposure to UVB upregulated matrix metalloproteinase-13 (MMP-13) and cyclooxygenase-2 (COX-2) expression, while consumption of RBS suppressed MMP-13 and COX-2 expression, as well as mitogen-activated protein kinase (MAPK) signaling pathways. These findings suggest that RBS could be a potential bioactive ingredient in nutricosmetics to inhibit wrinkle formation and water content loss via the suppression of COX-2 and MMP-13 expression.     

百令胶囊联合厄贝沙坦片对膜性肾病患者MMP-9, MMP-3和TIMP-1水平的影响

目的:探究百令胶囊联合厄贝沙坦片对膜性肾病患者基质金属蛋白酶-9、3和金属蛋白酶组织抑制物-1影响。方法:收集我院肾内科收治的膜性肾病患者98例,根据随机对照表分为对照组和试验组,每组49例。对照组给予厄贝沙坦片治疗,试验组联合百令胶囊治疗。对比分析两组患者的临床疗效、血清Scr、BUN、UA、Ccr、尿蛋白、MMP-9、MMP-3及TIMP-l水平以及不良反应的发生情况。结果:治疗后,对照组临床总有效率为81.63%,显著低于试验组的95.92%(P0.05)。两组治疗后血清Scr、BUN、UA、MMP-9、MMP-3、TIMP-l水平均显著降低,且试验组显著低于对照组(P0.05),Ccr水平升高,且试验组显著高于对照组(P0.05)。对照组不良反应发生率为10.20%,试验组为6.25%,差异无统计学意义(P0.05)。结论:百令胶囊联合厄贝沙坦片对膜性肾病患者的临床疗效显著,安全性较高,可能与其显著降低MMP-9、MMP-3和TIMP-1水平有关。     

慢性睡眠限制状态下大鼠髁突软骨MMP-1,MMP-13表达的变化

目的:探讨MMP-1,MMP-13在慢性睡眠限制引起大鼠髁突软骨结构变化中的表达变化及作用。方法:180只雄性Wistar大鼠随机分为3组(n=60):慢性睡眠限制组(CSR)、大平台组(LC)、笼养组(CON)。每组根据试验时间不同分别分为3个亚组(n=20):7天(7D)、14天(14D)、21天(21D)组。参考改良多平台法(MMPM)建立大鼠的慢性睡眠限制模型。通过HE染色观察大鼠髁突软骨的结构变化。通过免疫组化和实时定量PCR分别检测MMP-1和MMP-13的蛋白水平及m RNA水平的表达变化。结果:HE染色和扫描电镜结果显示,CSR组的大鼠髁突软骨出现了病理性的改变。与CON和LC组比较,CSR组MMP-1和MMP-13的m RNA转录和蛋白表达水平明显升高(P0.05)。结论:慢性睡眠限制能够引起大鼠颞下颌关节髁突软骨的病理性变化。MMP-1和MMP-13的表达水平的变化可能在大鼠髁突软骨病理性改变中起关键作用。     

基质金属蛋白酶及其抑制剂在肝纤维化中的表达变化

目的 观察肝纤维化形成过程中基质金属蛋白酶MMP-1及其抑制剂TIMP-1的表达变化,从细胞外基质降解代谢的角度研究四氯化碳(CCl4)中毒性肝纤维化发生的机制.方法 雄性Wistar大鼠20只,分为正常组和肝纤维化模型组.肝纤维化组采用CCl4、饮酒、高脂低蛋白饮食等复合病因刺激制备肝纤维化动物模型,造模时间为8周.实验结束后测定肝脏指数、血清透明质酸(HA)、谷丙转氨酶(ALT)及尿羟脯氨酸(HYP)排出量,光镜下观察肝组织纤维化程度,并用免疫组化SABC法检测肝组织中Ⅰ、Ⅲ型胶原蛋白及MMP-1、TIMP-1的表达,同时用荧光实时定量PCR(RT-PCR)的方法检测肝组织中MMP-1、TIMP-1 mRNA的表达.结果 与正常对照组比较,肝纤维化模型组大鼠肝脏指数、血清HA及ALT显著增高,尿羟脯氨酸的排出量明显增加,病理组织学检查发现肝组织内纤维结缔组织增生明显,有假小叶形成;免疫组化的结果显示肝组织内Ⅰ、Ⅲ型胶原蛋白、MMP-1及TIMP-1的表达较正常组显著增加.结论 肝组织中MMP-1及TIMP-1的表达变化可能是导致肝纤维化的重要机制之一.     

转录因子Ets-1与MMP-9在胃癌中的表达及临床意义

目的观察转录因子Ets-1和MMP-9在胃癌组织中的表达;探讨两者在胃癌浸润转移中的作用、相互关系及意义。方法采用免疫组织化学S-P法检测97例胃癌及癌旁组织、28例正常胃黏膜组织中Ets-1和MMP-9的表达。结果胃癌组织中Ets-1和MMP-9的阳性表达率分别为74.2%(72/97)、75.3%(73/97),均明显高于癌旁组织(40.2%、18.6%)及正常胃黏膜组织(17.9%、14.3%)(P0.01);而在癌旁组织及正常胃黏膜组织中两者的表达差异无显著性(P0.05)。Ets-1和MMP-9的阳性表达率在乳头状腺癌、管状腺癌及低分化腺癌与黏液癌之间差异有显著性(P0.01)。Ets-1和MMP-9的高表达与胃癌浸润深度、淋巴结转移及临床分期有关(P0.01),与性别、年龄、肿瘤大小及肿瘤位置均无关(P0.05)。Ets-1和MMP-9的表达成正相关(r=0.700,P0.01)。结论Ets-1和MMP-9高表达与胃癌的浸润、转移密切相关;通过上调MMP-9的表达,可能是Ets-1促进胃癌浸润转移的机制之一。     

嗜热菌Thermus sp.YBJ-1的分离和淀粉酶基因的克隆

从西藏热泉水样分离得到一株嗜热菌(YBJ-1),其16S rDNA(1511bp)序列与栖热菌(Thermus scotoductus ITI-252T)的同源性为98％。通过PCR技术将Thermus sp．YBJ-1的淀粉酶基因(amyT)全长开放阅读框克隆到T载体。分析表明,amyT的ORF全长为1767bp,编码588个氨基酸。推导的氨基酸序列与嗜热脂肪芽孢杆菌的阿尔法环糊精酶(Bacillus stearothermophilus alpha-eyclodextrinase)和栖热菌Thermus sp．IM6501的麦芽糖淀粉酶(Thermus sp．IM6501 mahogenic amylase)分别有99％和96％的同源性,与嗜热脂肪芽孢杆菌的新普鲁兰酶(neopullulanase)的同源性为81％。