Preparation of arsenic trioxide-loaded albuminutes immunonanospheres and its specific killing effect on bladder cancer cell in vitro
Background Recently, arsenic trioxide (As2O3) was considered as a novel anti-tumor agent. However, it showed severe toxicity effect on normal tissue at the same time. To improve its therapeutic efficacy and decrease its toxicity, we prepared arsenic trioxide-loaded albuminutes immuno-nanospheres [ A...
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| Veröffentlicht in: | Chinese medical journal 2005, Vol.118 (1), p.50-55 |
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| description | Background Recently, arsenic trioxide (As2O3) was considered as a novel anti-tumor agent. However, it showed severe toxicity effect on normal tissue at the same time. To improve its therapeutic efficacy and decrease its toxicity, we prepared arsenic trioxide-loaded albuminutes immuno-nanospheres [ As2O3-( HAS-NS)-BDI-1 ] targeted with nonoclonal antibody (McAb) BDI-1 and tested its specific killing effect against bladder cancer cell. Methods As2O3-HAS-NS was prepared by chemical cross-linking method. Monoclonal antibody BDI-1 was purified with ammonium sulphate sahingout and chromatography. Albuminutes microspheres were conjugated with McAb by SPDP cross-linking method. Concentration of As in As2O3-(HAS-NS)-BDI-1 and As2O3-HAS-NS was measured by atomic fluometry method. As2O3- (HAS-NS)-BDI-1 and its activity were detected by SDS-PAGE reduction electrophoresis, indirect immunofluorescence test, light microscope and scanning electron microscope observation. Acridine orange staining and tritiated thymidine (^3H-TdR) incorporation tests were used to indicate soecific killing activity of As2O3-(HAS-NS)-BDI-1 in vitro. Results In As2O3- (HAS-NS)-BDI-1 groups, we saw two protein bands in SDS-PAGE reduction electrophoresis. Albuminutes immuno-nanospheres were rounded with clear green fluorescence by immunofluorescence test. Under microscope, we observed that BIU-87 cells were covered with the As2O3-(HAS-NS)-BDI-1 and that As2O3- (HAS-NS)-BDI-1 moved with the BIU-87 cells. The albuminutes immunonanospheres were tightly junctioned with the BIU-87 cells. Specific killing activity of As2O3-(HAS-NS) -BDI-1 on bladder tumor cells was observed by acridine orange staining and ^3H-TdR incorporation assays. Conclusions As2O3- (HAS-NS)-BDI-1 might bind specifically against BIU-87 cells, thus leading to high activity of killing bladder tumor cells. |
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However, it showed severe toxicity effect on normal tissue at the same time. To improve its therapeutic efficacy and decrease its toxicity, we prepared arsenic trioxide-loaded albuminutes immuno-nanospheres [ As2O3-( HAS-NS)-BDI-1 ] targeted with nonoclonal antibody (McAb) BDI-1 and tested its specific killing effect against bladder cancer cell. Methods As2O3-HAS-NS was prepared by chemical cross-linking method. Monoclonal antibody BDI-1 was purified with ammonium sulphate sahingout and chromatography. Albuminutes microspheres were conjugated with McAb by SPDP cross-linking method. Concentration of As in As2O3-(HAS-NS)-BDI-1 and As2O3-HAS-NS was measured by atomic fluometry method. As2O3- (HAS-NS)-BDI-1 and its activity were detected by SDS-PAGE reduction electrophoresis, indirect immunofluorescence test, light microscope and scanning electron microscope observation. Acridine orange staining and tritiated thymidine (^3H-TdR) incorporation tests were used to indicate soecific killing activity of As2O3-(HAS-NS)-BDI-1 in vitro. Results In As2O3- (HAS-NS)-BDI-1 groups, we saw two protein bands in SDS-PAGE reduction electrophoresis. Albuminutes immuno-nanospheres were rounded with clear green fluorescence by immunofluorescence test. Under microscope, we observed that BIU-87 cells were covered with the As2O3-(HAS-NS)-BDI-1 and that As2O3- (HAS-NS)-BDI-1 moved with the BIU-87 cells. The albuminutes immunonanospheres were tightly junctioned with the BIU-87 cells. Specific killing activity of As2O3-(HAS-NS) -BDI-1 on bladder tumor cells was observed by acridine orange staining and ^3H-TdR incorporation assays. Conclusions As2O3- (HAS-NS)-BDI-1 might bind specifically against BIU-87 cells, thus leading to high activity of killing bladder tumor cells.</description><identifier>ISSN: 0366-6999</identifier><identifier>EISSN: 2542-5641</identifier><language>eng</language><subject>As2O3 ; 免疫沉淀反应 ; 白蛋白 ; 砷三氧化物 ; 膀胱肿瘤</subject><ispartof>Chinese medical journal, 2005, Vol.118 (1), p.50-55</ispartof><lds50>peer_reviewed</lds50><woscitedreferencessubscribed>false</woscitedreferencessubscribed></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Uhttp://image.cqvip.com/vip1000/qk/85656X/85656X.jpg</thumbnail><link.rule.ids>314,780,784,4024</link.rule.ids></links><search><creatorcontrib>ZHOUJie ZENGFu-qing LIChong TONGQiang-song GAOXiang XIEShu-sheng YULi-zhang</creatorcontrib><title>Preparation of arsenic trioxide-loaded albuminutes immunonanospheres and its specific killing effect on bladder cancer cell in vitro</title><title>Chinese medical journal</title><addtitle>Chinese Medical Journal</addtitle><description>Background Recently, arsenic trioxide (As2O3) was considered as a novel anti-tumor agent. However, it showed severe toxicity effect on normal tissue at the same time. To improve its therapeutic efficacy and decrease its toxicity, we prepared arsenic trioxide-loaded albuminutes immuno-nanospheres [ As2O3-( HAS-NS)-BDI-1 ] targeted with nonoclonal antibody (McAb) BDI-1 and tested its specific killing effect against bladder cancer cell. Methods As2O3-HAS-NS was prepared by chemical cross-linking method. Monoclonal antibody BDI-1 was purified with ammonium sulphate sahingout and chromatography. Albuminutes microspheres were conjugated with McAb by SPDP cross-linking method. Concentration of As in As2O3-(HAS-NS)-BDI-1 and As2O3-HAS-NS was measured by atomic fluometry method. As2O3- (HAS-NS)-BDI-1 and its activity were detected by SDS-PAGE reduction electrophoresis, indirect immunofluorescence test, light microscope and scanning electron microscope observation. Acridine orange staining and tritiated thymidine (^3H-TdR) incorporation tests were used to indicate soecific killing activity of As2O3-(HAS-NS)-BDI-1 in vitro. Results In As2O3- (HAS-NS)-BDI-1 groups, we saw two protein bands in SDS-PAGE reduction electrophoresis. Albuminutes immuno-nanospheres were rounded with clear green fluorescence by immunofluorescence test. Under microscope, we observed that BIU-87 cells were covered with the As2O3-(HAS-NS)-BDI-1 and that As2O3- (HAS-NS)-BDI-1 moved with the BIU-87 cells. The albuminutes immunonanospheres were tightly junctioned with the BIU-87 cells. Specific killing activity of As2O3-(HAS-NS) -BDI-1 on bladder tumor cells was observed by acridine orange staining and ^3H-TdR incorporation assays. Conclusions As2O3- (HAS-NS)-BDI-1 might bind specifically against BIU-87 cells, thus leading to high activity of killing bladder tumor cells.</description><subject>As2O3</subject><subject>免疫沉淀反应</subject><subject>白蛋白</subject><subject>砷三氧化物</subject><subject>膀胱肿瘤</subject><issn>0366-6999</issn><issn>2542-5641</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2005</creationdate><recordtype>article</recordtype><recordid>eNqNjMFKxDAURYMoWHX-4eG-0HaalK5FcenC_fCavMw8J33pJKn4AX64FfwAVwcu95wrVXW672pt-vZaVc3emNqM43ir7nL-aJpO68FU6vst0YIJC0eB6AFTJmELJXH8Ykd1iOjIAYZpnVnWQhl4nleJghLzcqK0LSgOuGTIC1n2m37mEFiOQN6TLbC1p4DOUQKLYn9BIQALfHJJ8UHdeAyZdn-8V48vz-9Pr7U9RTlettBhQnv2HOjQtmZo-0Hv_3X6AQS4U9w</recordid><startdate>2005</startdate><enddate>2005</enddate><creator>ZHOUJie ZENGFu-qing LIChong TONGQiang-song GAOXiang XIEShu-sheng YULi-zhang</creator><scope>2RA</scope><scope>92L</scope><scope>CQIGP</scope><scope>W91</scope><scope>~WA</scope></search><sort><creationdate>2005</creationdate><title>Preparation of arsenic trioxide-loaded albuminutes immunonanospheres and its specific killing effect on bladder cancer cell in vitro</title><author>ZHOUJie ZENGFu-qing LIChong TONGQiang-song GAOXiang XIEShu-sheng YULi-zhang</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-chongqing_backfile_116714753</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2005</creationdate><topic>As2O3</topic><topic>免疫沉淀反应</topic><topic>白蛋白</topic><topic>砷三氧化物</topic><topic>膀胱肿瘤</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>ZHOUJie ZENGFu-qing LIChong TONGQiang-song GAOXiang XIEShu-sheng YULi-zhang</creatorcontrib><collection>中文科技期刊数据库</collection><collection>中文科技期刊数据库-CALIS站点</collection><collection>中文科技期刊数据库-7.0平台</collection><collection>中文科技期刊数据库-医药卫生</collection><collection>中文科技期刊数据库- 镜像站点</collection><jtitle>Chinese medical journal</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>ZHOUJie ZENGFu-qing LIChong TONGQiang-song GAOXiang XIEShu-sheng YULi-zhang</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Preparation of arsenic trioxide-loaded albuminutes immunonanospheres and its specific killing effect on bladder cancer cell in vitro</atitle><jtitle>Chinese medical journal</jtitle><addtitle>Chinese Medical Journal</addtitle><date>2005</date><risdate>2005</risdate><volume>118</volume><issue>1</issue><spage>50</spage><epage>55</epage><pages>50-55</pages><issn>0366-6999</issn><eissn>2542-5641</eissn><abstract>Background Recently, arsenic trioxide (As2O3) was considered as a novel anti-tumor agent. However, it showed severe toxicity effect on normal tissue at the same time. To improve its therapeutic efficacy and decrease its toxicity, we prepared arsenic trioxide-loaded albuminutes immuno-nanospheres [ As2O3-( HAS-NS)-BDI-1 ] targeted with nonoclonal antibody (McAb) BDI-1 and tested its specific killing effect against bladder cancer cell. Methods As2O3-HAS-NS was prepared by chemical cross-linking method. Monoclonal antibody BDI-1 was purified with ammonium sulphate sahingout and chromatography. Albuminutes microspheres were conjugated with McAb by SPDP cross-linking method. Concentration of As in As2O3-(HAS-NS)-BDI-1 and As2O3-HAS-NS was measured by atomic fluometry method. As2O3- (HAS-NS)-BDI-1 and its activity were detected by SDS-PAGE reduction electrophoresis, indirect immunofluorescence test, light microscope and scanning electron microscope observation. Acridine orange staining and tritiated thymidine (^3H-TdR) incorporation tests were used to indicate soecific killing activity of As2O3-(HAS-NS)-BDI-1 in vitro. Results In As2O3- (HAS-NS)-BDI-1 groups, we saw two protein bands in SDS-PAGE reduction electrophoresis. Albuminutes immuno-nanospheres were rounded with clear green fluorescence by immunofluorescence test. Under microscope, we observed that BIU-87 cells were covered with the As2O3-(HAS-NS)-BDI-1 and that As2O3- (HAS-NS)-BDI-1 moved with the BIU-87 cells. The albuminutes immunonanospheres were tightly junctioned with the BIU-87 cells. Specific killing activity of As2O3-(HAS-NS) -BDI-1 on bladder tumor cells was observed by acridine orange staining and ^3H-TdR incorporation assays. Conclusions As2O3- (HAS-NS)-BDI-1 might bind specifically against BIU-87 cells, thus leading to high activity of killing bladder tumor cells.</abstract></addata></record> |
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| subjects | As2O3 免疫沉淀反应 白蛋白 砷三氧化物 膀胱肿瘤 |
| title | Preparation of arsenic trioxide-loaded albuminutes immunonanospheres and its specific killing effect on bladder cancer cell in vitro |
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