公开(公告)号：US20120108803A1

公开(公告)日：2012-05-03

申请号：US13319885

申请日：2010-05-13

申请人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

发明人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

IPC分类号： C07H21/02 ,  C07F7/10 ,  B82Y5/00

CPC分类号： A61K47/48215 ,  A61K9/1075 ,  A61K47/34 ,  A61K47/60 ,  B82Y5/00 ,  C07F7/0836 ,  C07H21/02 ,  C08G65/3356 ,  C12N15/111 ,  C12N15/113 ,  C12N2310/11 ,  C12N2310/14 ,  C12N2310/351 ,  C12N2310/3515 ,  C12N2320/30 ,  C12N2320/51 ,  Y10S977/773 ,  Y10S977/906

摘要： Provided are an siRNA-polymer conjugate, and a method for preparing the same, and more specifically, to a hybrid conjugate formed by covalently bonding siRNA and a polymeric compound for improving the in vivo stability of siRNA, and to a preparation method of the hybrid conjugate. The conjugate of the present invention can improve the in vivo stability of siRNA, thereby achieving an efficient delivery of therapeutic siRNA into cells and exhibiting the activity of siRNA even with a small dose of a relative low concentration. Therefore, the conjugate can advantageously be used as not only an siRNA treatment tool for cancers and other infectious disease, but also a novel type siRNA delivery system.

摘要翻译： 提供了siRNA-聚合物缀合物及其制备方法，更具体地说，涉及通过共价键合siRNA和高分子化合物形成的用于提高siRNA体内稳定性的杂合偶联物，以及该混合物的制备方法 缀合物。 本发明的缀合物可以提高siRNA的体内稳定性，从而实现治疗性siRNA有效递送到细胞中，并且即使用相对低浓度的小剂量也显示出siRNA的活性。 因此，缀合物不仅可以有效地用作癌症和其它感染性疾病的siRNA治疗工具，还可以用作新型siRNA递送系统。

公开(公告)号：US08779114B2

公开(公告)日：2014-07-15

申请号：US13319885

申请日：2010-05-13

申请人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

发明人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

IPC分类号： A61K47/00 ,  A61K9/107 ,  A61K47/48 ,  A61K47/34

CPC分类号： A61K47/48215 ,  A61K9/1075 ,  A61K47/34 ,  A61K47/60 ,  B82Y5/00 ,  C07F7/0836 ,  C07H21/02 ,  C08G65/3356 ,  C12N15/111 ,  C12N15/113 ,  C12N2310/11 ,  C12N2310/14 ,  C12N2310/351 ,  C12N2310/3515 ,  C12N2320/30 ,  C12N2320/51 ,  Y10S977/773 ,  Y10S977/906

摘要： Provided are an siRNA-polymer conjugate, and a method for preparing the same, and more specifically, to a hybrid conjugate formed by covalently bonding siRNA and a polymeric compound for improving the in vivo stability of siRNA, and to a preparation method of the hybrid conjugate. The conjugate of the present invention can improve the in vivo stability of siRNA, thereby achieving an efficient delivery of therapeutic siRNA into cells and exhibiting the activity of siRNA even with a small dose of a relative low concentration. Therefore, the conjugate can advantageously be used as not only an siRNA treatment tool for cancers and other infectious disease, but also a novel type siRNA delivery system.

摘要翻译： 提供了siRNA-聚合物缀合物及其制备方法，更具体地，涉及通过共价键合siRNA和高分子化合物形成的用于提高siRNA体内稳定性的杂合偶联物，以及该混合物的制备方法 缀合物。 本发明的缀合物可以提高siRNA的体内稳定性，从而实现治疗性siRNA有效递送到细胞中，并且即使用相对低浓度的小剂量也显示出siRNA的活性。 因此，缀合物不仅可以有效地用作癌症和其它感染性疾病的siRNA治疗工具，还可以用作新型siRNA递送系统。

公开(公告)号：US20130096288A1

公开(公告)日：2013-04-18

申请号：US13613071

申请日：2012-09-13

申请人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

发明人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

IPC分类号： C08G65/335

CPC分类号： A61K47/48215 ,  A61K9/1075 ,  A61K47/34 ,  A61K47/60 ,  B82Y5/00 ,  C07F7/0836 ,  C07H21/02 ,  C08G65/3356 ,  C12N15/111 ,  C12N15/113 ,  C12N2310/11 ,  C12N2310/14 ,  C12N2310/351 ,  C12N2310/3515 ,  C12N2320/30 ,  C12N2320/51 ,  Y10S977/773 ,  Y10S977/906

摘要： Provided are an siRNA-polymer conjugate, and a method for preparing the same, and more specifically, to a hybrid conjugate formed by covalently bonding siRNA and a polymeric compound for improving the in vivo stability of siRNA, and to a preparation method of the hybrid conjugate. The conjugate of the present invention can improve the in vivo stability of siRNA, thereby achieving an efficient delivery of therapeutic siRNA into cells and exhibiting the activity of siRNA even with a small dose of a relative low concentration. Therefore, the conjugate can advantageously be used as not only an siRNA treatment tool for cancers and other infectious disease, but also a novel type siRNA delivery system.

公开(公告)号：US08772472B2

公开(公告)日：2014-07-08

申请号：US13613071

申请日：2012-09-13

申请人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

发明人： Bo Ram Han ,  Han Oh Park ,  Mi Sik Shin ,  Sam Young Lee

IPC分类号： A61K47/00 ,  A61K9/107 ,  A61K47/48 ,  A61K47/34

CPC分类号： A61K47/48215 ,  A61K9/1075 ,  A61K47/34 ,  A61K47/60 ,  B82Y5/00 ,  C07F7/0836 ,  C07H21/02 ,  C08G65/3356 ,  C12N15/111 ,  C12N15/113 ,  C12N2310/11 ,  C12N2310/14 ,  C12N2310/351 ,  C12N2310/3515 ,  C12N2320/30 ,  C12N2320/51 ,  Y10S977/773 ,  Y10S977/906

摘要： Provided are an siRNA-polymer conjugate, and a method for preparing the same, and more specifically, to a hybrid conjugate formed by covalently bonding siRNA and a polymeric compound for improving the in vivo stability of siRNA, and to a preparation method of the hybrid conjugate. The conjugate of the present invention can improve the in vivo stability of siRNA, thereby achieving an efficient delivery of therapeutic siRNA into cells and exhibiting the activity of siRNA even with a small dose of a relative low concentration. Therefore, the conjugate can advantageously be used as not only an siRNA treatment tool for cancers and other infectious disease, but also a novel type siRNA delivery system.

摘要翻译： 提供了siRNA-聚合物缀合物及其制备方法，更具体地，涉及通过共价键合siRNA和高分子化合物形成的用于提高siRNA体内稳定性的杂合偶联物，以及该混合物的制备方法 缀合物。 本发明的缀合物可以提高siRNA的体内稳定性，从而实现治疗性siRNA有效递送到细胞中，并且即使用相对低浓度的小剂量也显示出siRNA的活性。 因此，缀合物不仅可以有效地用作癌症和其它感染性疾病的siRNA治疗工具，还可以用作新型siRNA递送系统。

公开(公告)号：US09273306B2

公开(公告)日：2016-03-01

申请号：US13885556

申请日：2011-11-18

申请人： Han Oh Park ,  Byung Rae Jeong ,  Kwon Sic Kim

发明人： Han Oh Park ,  Byung Rae Jeong ,  Kwon Sic Kim

IPC分类号： C12Q1/68 ,  B01L3/00 ,  C12N15/10

CPC分类号： C12N15/1013 ,  C12Q1/68

摘要： Disclosed is an automatic nucleic acid purification apparatus which can prevent pollution due to aerosol generated from a biological sample containing high concentration target nucleic acid when the biological sample containing the high concentration target nucleic acid is mixed with other biological sample containing low concentration target nucleic acid or not containing the target nucleic acid. Further, disclosed is an automatic nucleic acid purification apparatus which can be applied to all kinds of nucleic acid purification equipments for purifying a plurality of biological samples using a magnet rode or a multi-pipette block moving in two or three axial directions, and which can minimize pollution due to the aerosol generated from the biological sample containing high concentration target nucleic acid and also can obtain accurate results.

摘要翻译： 公开了一种自动核酸纯化装置，当含有高浓度靶核酸的生物样品与含有低浓度靶核酸的其他生物样品混合时，可以防止由含有高浓度靶核酸的生物样品产生的气溶胶引起的污染，或 不含靶核酸。 此外，公开了一种自动核酸纯化装置，其可以应用于使用磁珠或多个移液管块在两个或三个轴向移动的多个生物样品的各种核酸纯化设备，并且其可以 尽可能减少由含有高浓度靶核酸的生物样品产生的气溶胶引起的污染，并可获得准确的结果。

公开(公告)号：US09163272B2

公开(公告)日：2015-10-20

申请号：US14238908

申请日：2012-08-23

申请人： Han Oh Park ,  You Sang Cho ,  Jun Ho Jung ,  Ji Won Han ,  Nam Il Kim

发明人： Han Oh Park ,  You Sang Cho ,  Jun Ho Jung ,  Ji Won Han ,  Nam Il Kim

IPC分类号： C07K1/22 ,  C07K1/00 ,  C07K1/14 ,  C12P21/00 ,  B01J19/00 ,  C12P21/02

CPC分类号： C12P21/00 ,  B01J19/0046 ,  B01J2219/00315 ,  B01J2219/00364 ,  B01J2219/00459 ,  B01J2219/00495 ,  C07K1/22 ,  C12P21/02

摘要： Provided is a method of protein synthesis. The method of protein synthesis according to the present invention uses an automatic biological material purification apparatus including: a well plate kit; a heating part; and a magnetic field applying part, such that a plurality of target proteins may be more quickly and simply obtained as compared to target proteins obtained by using the existing method for expressing/purifying proteins through conventional cell culture, and a reproducible synthesis efficiency on the same proteins may be obtained due to no deviation between reaction wells.

摘要翻译： 提供蛋白质合成的方法。 根据本发明的蛋白质合成方法使用自动生物材料净化装置，其包括：孔板试剂盒; 加热部件 和磁场施加部分，使得与通过使用现有的通过常规细胞培养表达/纯化蛋白质的方法获得的靶蛋白相比，可以更快速和简单地获得多个靶蛋白质，并且可以在其上产生可再现的合成效率 由于反应孔之间没有偏差，可以获得蛋白质。

公开(公告)号：US20140212919A1

公开(公告)日：2014-07-31

申请号：US14238908

申请日：2012-08-23

申请人： Han Oh Park ,  You Sang Cho ,  Jun Ho Jung ,  Ji Won Han ,  Nam Il Kim

发明人： Han Oh Park ,  You Sang Cho ,  Jun Ho Jung ,  Ji Won Han ,  Nam Il Kim

IPC分类号： C12P21/00

CPC分类号： C12P21/00 ,  B01J19/0046 ,  B01J2219/00315 ,  B01J2219/00364 ,  B01J2219/00459 ,  B01J2219/00495 ,  C07K1/22 ,  C12P21/02

摘要： Provided is a method of protein synthesis. The method of protein synthesis according to the present invention uses an automatic biological material purification apparatus including: a well plate kit; a heating part; and a magnetic field applying part, such that a plurality of target proteins may be more quickly and simply obtained as compared to target proteins obtained by using the existing method for expressing/purifying proteins through conventional cell culture, and a reproducible synthesis efficiency on the same proteins may be obtained due to no deviation between reaction wells.

摘要翻译： 提供蛋白质合成的方法。 根据本发明的蛋白质合成方法使用自动生物材料净化装置，其包括：孔板试剂盒; 加热部件 和磁场施加部分，使得与通过使用现有的通过常规细胞培养表达/纯化蛋白质的方法获得的靶蛋白相比，可以更快速和简单地获得多个靶蛋白质，并且可以在其上产生可再现的合成效率 由于反应孔之间没有偏差，可以获得蛋白质。

公开(公告)号：US20140087377A1

公开(公告)日：2014-03-27

申请号：US14005213

申请日：2012-03-13

申请人： Han Oh Park ,  Jung Young Choi ,  Eun Su Han ,  Gu Young Song ,  Won Seok Jang

发明人： Han Oh Park ,  Jung Young Choi ,  Eun Su Han ,  Gu Young Song ,  Won Seok Jang

IPC分类号： C12Q1/68

CPC分类号： C12Q1/6816 ,  C12Q1/6818 ,  C12Q2521/327 ,  C12Q2525/121 ,  C12Q2563/185

摘要： The present invention relates to a method of identifying nucleic acid-containing object, more precisely a method of identifying nucleic acid-containing object which comprises the following steps: (1) preparing nucleic acid-containing object having the nucleotide sequence complementary to the nucleotide sequence of RNA-dual probe; (2) reacting the nucleic acid included in the object with the buffer containing the RNA-dual probe conjugated with a reporter and a quencher respectively and RNase; and (3) detecting fluorescence generated from the reporter. The method of identifying an object of the present invention provides labeling sensitivity 100 times as high as that of the conventional method using sequencing or labeling with fluorescent materials, takes advantages of shorter analysis time, facilitates different labeling on a variety of products according to fluorescent materials, and makes possible unlimited product administration by product group and batch in real production process by differentiating the nucleotide sequence of each oligonucleotide.

摘要翻译： 本发明涉及鉴定含核酸物质的方法，更准确地说，一种鉴定含核酸物质的方法，包括以下步骤：（1）制备具有与核苷酸序列互补的核苷酸序列的含核酸物质 的RNA双探针; （2）将包含在物体中的核酸与分别与报告子和猝灭剂结合的RNA双重探针的缓冲液和RNase分别反应; 和（3）检测从报告物产生的荧光。 识别本发明的目的的方法提供了使用荧光材料进行测序或标记的常规方法的100倍的标签灵敏度，具有较短的分析时间的优点，便于根据荧光材料对各种产品进行不同的标记 并通过区分每个寡核苷酸的核苷酸序列，在实际生产过程中使产品组和批次无限制地进行产品管理。

公开(公告)号：US20130115686A1

公开(公告)日：2013-05-09

申请号：US13810534

申请日：2011-06-01

申请人： Han Oh Park ,  Gu Young Song ,  Jung A Bae

发明人： Han Oh Park ,  Gu Young Song ,  Jung A Bae

IPC分类号： G01N21/64

CPC分类号： B01L3/502 ,  B01L3/50255 ,  B01L3/50851 ,  B01L2200/12 ,  B01L2200/16 ,  B01L2300/044 ,  B01L2300/048 ,  B01L2300/0681 ,  B01L2300/0829 ,  B01L2400/0409 ,  B01L2400/049 ,  C12M23/12 ,  G01N21/6454 ,  Y10T29/51 ,  Y10T137/0402

摘要： The present invention relates to a micro chamber plate, and more particularly, to an analytic micro chamber plate in which a plurality of reaction solutions including a primer or probe selectively reacting with a nucleic acid react with each other without cross-contamination to measure and analyze a fluorescence level in real-time so as to analyze biological sample solution including a large amount of nucleic acids. Also, the present invention relates to a method of manufacturing the analytic chamber plate. Also, the present invention relates to a method of manufacturing a micro chamber plate with a built-in sample used for manufacturing the analytic chamber plate. Also, the present invention relates to an apparatus set for manufacturing the micro chamber plate with a built-in sample.

摘要翻译： 本发明涉及一种微室板，更具体地说，涉及一种分析微室板，其中包括选择性与核酸反应的引物或探针的多个反应溶液彼此反应而没有交叉污染以测量和分析 荧光水平实时分析生物样品溶液，包括大量的核酸。 此外，本发明涉及一种制造分析室板的方法。 此外，本发明涉及一种制造具有用于制造分析室板的内置样品的微室板的方法。 此外，本发明涉及一种用于制造具有内置样品的微室板的装置。

公开(公告)号：US20130230860A1

公开(公告)日：2013-09-05

申请号：US13881900

申请日：2011-10-27

申请人： Han Oh Park ,  Kwon Sic Kim ,  Yang Won Lee ,  Jin II Lee ,  Byung Rae Jeong ,  Jong Hoon Kim

发明人： Han Oh Park ,  Kwon Sic Kim ,  Yang Won Lee ,  Jin II Lee ,  Byung Rae Jeong ,  Jong Hoon Kim

IPC分类号： C12Q1/68

CPC分类号： C12Q1/686 ,  B01L3/0227 ,  B01L3/0234 ,  B01L7/52 ,  B01L2300/0829 ,  B01L2300/1805 ,  B01L2400/0478 ,  B03C1/01 ,  B03C1/288 ,  B03C2201/26 ,  C12Q1/02 ,  C12Q1/6844 ,  G01N35/0098 ,  G01N35/028 ,  G01N2035/0425 ,  G01N2035/0465

摘要： The present invention relates to an automatic real-time quantitative amplification system which can perform analysis of various biological samples, and more particularly to an automatic real-time quantitative amplification system in which a plurality of decks for respectively accommodating biological samples are put in a deck storing/transferring device, whereby it is possible to automatically analyze an amount or existence of a target substance containing a target nucleic acid in the biologic sample, such as a particular gene, a particular, a particular pathogenic bacterium and a particular protein, by amplifying the target nucleic acid purified by some processes of purification, purification after culture, or purification after reaction of the target substance contained in the bio-logical sample and then checking an amount of the amplified target nucleic acid.

摘要翻译： 本发明涉及一种能够对各种生物样品进行分析的自动实时定量放大系统，更具体地涉及一种自动实时定量放大系统，其中将用于分别容纳生物样品的多个甲板放入甲板 存储/转移装置，从而可以通过扩增生物样品中特定的基因，特定的，特定的致病菌和特定的蛋白质自动分析含有靶核酸的目标物质的量或存在 通过纯化的一些方法，培养后的纯化，或者生物样品中包含的目标物质的反应后的纯化，然后检查扩增的目标核酸的量来纯化靶核酸。