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公开(公告)号:US5874984A
公开(公告)日:1999-02-23
申请号:US495592
申请日:1995-08-02
申请人: Christian Scholz , Manfred Wiedemer
发明人: Christian Scholz , Manfred Wiedemer
CPC分类号: H01L27/153 , B41J2/45 , H01L2224/05553 , H01L2224/05554 , H01L2224/48091 , H01L2224/48137 , H01L2224/49175 , H01L27/156
摘要: An optical character generator for an electrographic printer has a plurality of monolithic circuits (11) which are arranged on a carrier (10) and have LEDs (12) which are integrated in the circuits and can be driven individually. The monolithic circuits (11) include a monolithically integrated photodiode drive combination, in the case of which both the associated LEDs (12) and the drive circuit (13), possibly including a BUS circuit (14) for the LEDs (12), are integrated in a monolithic circuit (11). The monolithic circuits are constructed using thin-film technology from III-V semiconductor material, preferably GaAs.
摘要翻译: PCT No.PCT / DE94 / 00097 Sec。 371日期:1995年8月2日 102(e)日期1995年8月2日PCT 1994年2月1日PCT PCT。 出版物WO94 / 18704 日期1994年8月18日用于电印机的光学字符发生器具有多个单片电路(11),其布置在载体(10)上并具有集成在电路中并可单独驱动的LED(12)。 在其中可能包括用于LED(12)的BUS电路(14)的相关联的LED(12)和驱动电路(13)两者都是相同的情况下,单片电路(11)包括单片集成的光电二极管驱动组合 集成在单片电路(11)中。 使用来自III-V半导体材料(优选GaAs)的薄膜技术构建单片电路。
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公开(公告)号:US20120308994A1
公开(公告)日:2012-12-06
申请号:US13569353
申请日:2012-08-08
IPC分类号: G01N21/76 , G01N33/569
CPC分类号: C12N15/62 , C12N9/90 , G01N33/536 , G01N33/54393 , Y02A50/57
摘要: Disclosed are a recombinant DNA molecule encoding a fusion protein comprising a SlpA chaperone and a target polypeptide wherein human FK506 binding proteins (FKBPs) are excluded as target polypeptides, a corresponding expression vector encoding said fusion protein as well as host cells transformed with said expression vector. Also disclosed are a method for producing the fusion protein, a recombinantly produced fusion protein comprising a SlpA chaperone and a target polypeptide. A further aspect of the invention is the use of the recombinantly produced fusion protein, and a reagent kit containing a recombinantly produced fusion protein comprising a SlpA chaperone and a target polypeptide.
摘要翻译: 公开了编码包含SlpA伴侣和靶多肽的融合蛋白的重组DNA分子,其中人FK506结合蛋白(FKBP)被排除为靶多肽,编码所述融合蛋白的相应表达载体以及用所述表达载体转化的宿主细胞 。 还公开了产生融合蛋白的方法,重组产生的包含SlpA伴侣和靶多肽的融合蛋白。 本发明的另一方面是使用重组产生的融合蛋白,以及含有重组产生的包含SlpA伴侣和靶多肽的融合蛋白的试剂盒。
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63.发明申请FUSION PROTEIN COMPRISING AN E. COLI CHAPERONE PROTEIN AND A HUMAN CHAPERONE PROTEIN 有权包含大肠杆菌蛋白和蛋白质的融合蛋白公开(公告)号:US20110189754A1
公开(公告)日:2011-08-04
申请号:US13083903
申请日:2011-04-11
CPC分类号: C12N9/90 , C07K2319/35
摘要: The invention discloses the cloning, expression and uses of a chimeric fusion protein with superior chaperone and folding activities compared to the wild type chaperones. This invention relates to a chimeric fusion protein encoded by a recombinant DNA molecule containing nucleotide sequences coding for a polypeptide binding segment of a non-human chaperone protein and nucleotide sequences coding for an FK506 binding protein (FKBP) or an FK506-binding-protein-like domain (FKBP-like domain). In particular, this invention relates to a chimeric fusion protein encoded by a recombinant DNA molecule containing nucleotide sequences coding for a polypeptide binding segment of a non-human chaperone protein and nucleotide sequences coding for a human FKBP type peptidyl-prolyl-cis/trans isomerase (PPIase), methods of producing these chimeric fusion proteins and their uses as folding helpers in the production of other proteins and in the process of the production of vaccines or pharmaceuticals, and as folding helpers for performing immunoassays.
摘要翻译: 本发明公开了与野生型伴侣相比,具有优异的伴侣和折叠活性的嵌合融合蛋白的克隆,表达和用途。 本发明涉及由含有编码非人伴侣蛋白多肽结合片段的核苷酸序列的重组DNA分子编码的嵌合融合蛋白和编码FK506结合蛋白(FKBP)或FK506-结合蛋白 - 像域(FKBP样域)。 特别地,本发明涉及由包含编码非人伴侣蛋白多肽结合片段的核苷酸序列的重组DNA分子编码的嵌合融合蛋白和编码人FKBP型肽基 - 脯氨酰 - 顺/反异构酶的核苷酸序列 (PPIase),生产这些嵌合融合蛋白的方法及其在生产其他蛋白质和疫苗或药物生产过程中作为折叠助剂的用途,以及用于进行免疫测定的折叠助剂。
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公开(公告)号:USD612841S1
公开(公告)日:2010-03-30
申请号:US29343757
申请日:2009-09-18
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公开(公告)号:US20090042212A1
公开(公告)日:2009-02-12
申请号:US12104751
申请日:2008-04-17
IPC分类号: G01N33/53 , C07K7/00 , C07K14/00 , C12N15/11 , C12N15/00 , C12N1/20 , C12P21/04 , G01N33/566
CPC分类号: G01N33/6854 , C07K14/20 , C07K14/245 , C07K14/45 , C07K14/47 , C07K2319/70 , C12N15/62 , C12N2710/16122 , C12N2710/16134 , G01N2333/02 , G01N2333/035 , G01N2333/04 , G01N2333/045 , G01N2333/05 , G01N2333/19 , G01N2333/45
摘要: The present invention relates to fusion proteins: suitable as test antigens in the detection of infections with pathogens, particularly of primary infections with pathogens. Further, the invention relates to methods for detecting and differentially determining antibodies, particularly IgM antibodies resulting from an infection with a pathogenic organism. Furthermore, test reagents for carrying out these methods are provided.
摘要翻译: 本发明涉及融合蛋白:适合作为检测病原体感染的试验抗原,特别是病原体的初次感染。 此外,本发明涉及用于检测和差异测定抗体的方法,特别是由致病性生物体的感染产生的IgM抗体。 此外,提供了用于实施这些方法的测试试剂。
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66.发明申请Methods for producing fusion polypeptides or enhancing expression of fusion polypeptides 有权用于产生融合多肽或增强融合多肽表达的方法公开(公告)号:US20090028893A1
公开(公告)日:2009-01-29
申请号:US11786847
申请日:2007-04-13
申请人: Christian Scholz , Herbert Andres , Elke Faatz , Alfred Engel , Urban Schmitt , Ariuna Bazarsuren , Peter Schaarschmidt
发明人: Christian Scholz , Herbert Andres , Elke Faatz , Alfred Engel , Urban Schmitt , Ariuna Bazarsuren , Peter Schaarschmidt
CPC分类号: G01N33/56988 , A61K39/00 , A61K47/64 , C07K14/005 , C07K2319/00 , C12N9/90 , C12N2740/16122 , G01N33/54306 , G01N33/56911 , G01N33/56983 , G01N2333/005 , G01N2333/16 , G01N2333/195 , G01N2469/20
摘要: The present invention relates to the cloning and expression of foreign protein or polypeptides in bacteria, such as Escherichia coli. In particular, this invention relates to expression tools comprising a FKBP-type peptidyl prolyl isomerase selected from the group consisting of FkpA, SlyD, and trigger factor; methods of recombinant protein expression, the recombinant polypeptides thus obtained, as well as to the use of such polypeptides.
摘要翻译: 本发明涉及在细菌如大肠杆菌中克隆和表达外源蛋白质或多肽。 特别地,本发明涉及包含选自FkpA,SlyD和触发因子的FKBP型肽基脯氨酰异构酶的表达工具; 重组蛋白表达的方法,如此获得的重组多肽,以及这些多肽的用途。
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公开(公告)号:US20070154883A1
公开(公告)日:2007-07-05
申请号:US11584887
申请日:2006-10-23
申请人: Barbara Upmeier , Ralf Bollhagen , Alfred Engel , Elke Faatz , Peter Schaarschmidt , Christian Scholz , Toralf Zarnt
发明人: Barbara Upmeier , Ralf Bollhagen , Alfred Engel , Elke Faatz , Peter Schaarschmidt , Christian Scholz , Toralf Zarnt
IPC分类号: C12Q1/70
CPC分类号: C07K14/005 , C07K2319/35 , C12N2770/36222 , Y10S530/826
摘要: The invention disclosed relates to a soluble rubella E1 antigen and variants of this peptide characterized by lacking at the C-terminal end at least the transmembrane region and the anchor segment as well as at least the amino acids 143 to 164 and containing at least the region spanning the disulfide bridges Cys 349-Cys 352 and Cys 368-401 whereas the N-terminus (Cys 349) of this region contains additionally at least 15 amino acids and/or the C-terminus (Cys 401) of this region contains additionally at least 8 amino acids of the adjacent rubella E1 antigen sequence. Also described are a recombinant DNA molecule encoding the rubella E1 antigen and variants which are recombinantly expressed as a chaperone fusion protein, refolded into a soluble and immunoreactive conformation, and further used for the serological detection of anti-rubella antibodies. In addition, also disclosed is a method for the detection, determination and quantification of anti-rubella antibodies of IgG and/or IgM subclass in a sample wherein the rubella E1 antigen is used as a capture reagent and/or binding partner for the antibodies.
摘要翻译: 所公开的本发明涉及可溶性风疹E1抗原和该肽的变体,其特征在于至少在C-末端缺少至少跨膜区和锚段以及至少氨基酸143至164并且至少含有该区域 跨越二硫键Cys 349-Cys 352和Cys 368-401,而该区域的N末端(Cys 349)另外包含至少15个氨基酸和/或该区域的C末端(Cys 401) 相邻风疹E1抗原序列的至少8个氨基酸。 还描述了编码风疹E1抗原的重组DNA分子和重组表达为伴侣融合蛋白的变体,重新折叠成可溶性和免疫反应性构象,并进一步用于抗风疹抗体的血清学检测。 此外,还公开了用于检测,测定和定量样品中IgG和/或IgM亚类的抗风疹抗体的方法,其中所述风疹E1抗原用作抗体的捕获试剂和/或结合配偶体。
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68.发明授权公开(公告)号:US07016620B2
公开(公告)日:2006-03-21
申请号:US10486372
申请日:2002-07-24
申请人: Volkhard Maess , Hans Winter , Christian Scholz
发明人: Volkhard Maess , Hans Winter , Christian Scholz
IPC分类号: G03G15/043
CPC分类号: G03G15/0855 , G03G15/5041 , G03G2215/00042
摘要: In a method and device to control a print process in a printer or copier, with a character generator generating a latent print image and a latent toner marking on an image carrier. An exposure energy per unit area for the generation of the latent toner marking is decreased in comparison to an energy per unit area for generation of the latent print image. The latent print image and the latent toner marking are developed with toner in the developer station. An optical reflection sensor determines color density of the developed toner marking. Toner concentration is adjusted in a developer station dependent on a signal of the reflection sensor.
摘要翻译: 在用于控制打印机或复印机中的打印处理的方法和装置中,在图像载体上产生潜在打印图像和潜在墨粉标记的字符发生器。 潜在调色剂标记的产生的每单位面积的曝光能量相对于潜像印刷图像的每单位面积的能量而降低。 在显影剂站中用调色剂显影潜影图像和潜在调色剂标记。 光学反射传感器确定显影的调色剂标记的色彩浓度。 取决于反射传感器的信号,在显影剂站中调节调色剂浓度。
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69.发明授权Soluble complexes of target proteins and peptidyl prolyl isomerase chaperones and methods of making and using them 有权靶蛋白和肽基脯氨酰异构酶伴侣的可溶性复合物及其制备和使用方法公开(公告)号:US06962982B2
公开(公告)日:2005-11-08
申请号:US10179905
申请日:2002-06-24
申请人: Christian Scholz , Herbert Andres , Elke Faatz , Alfred Engel , Dorothea Sizmann
发明人: Christian Scholz , Herbert Andres , Elke Faatz , Alfred Engel , Dorothea Sizmann
IPC分类号: A61K39/00 , A61K47/48 , C07K14/16 , C12N9/90 , G01N33/543 , G01N33/569 , A61K38/24 , C07K14/00
CPC分类号: G01N33/56988 , A61K39/00 , A61K47/64 , C07K14/005 , C07K2319/00 , C12N9/90 , C12N2740/16122 , G01N33/54306 , G01N33/56911 , G01N33/56983 , G01N2333/005 , G01N2333/16 , G01N2333/195 , G01N2469/20 , G01N2800/2821
摘要: The present invention relates to the diagnosis of HIV infections. It especially teaches the production of a soluble retroviral surface glycoprotein- (or transmembrane glycoprotein)-chaperone complex and the advantageous use of a chaperone-antigen complex especially in the detection of antibodies to HIV in immunoassays, preferably according to the double antigen bridge concept, or as an immunogen. The invention also discloses soluble complexes comprising a variant of HIV-1 gp41 or a variant of HIV-2 gp36, respectively, and a chaperone selected from the peptidyl-prolyl-isomerase class of chaperones. Variants comprising specific amino-acid substitutions in the N-helical domain of HIV-1 gp41 or of HIV-2 gp36, respectively, are also described.
摘要翻译: 本发明涉及HIV感染的诊断。 特别是教导了可溶性逆转录病毒表面糖蛋白(或跨膜糖蛋白) - 辅助复合物的产生,并且优选地根据双抗原桥概念,优选使用伴侣 - 抗原复合物,特别是在免疫测定中检测HIV抗体中, 或作为免疫原。 本发明还公开了分别包含HIV-1 gp41的变体或HIV-2 gp36的变体的可溶性复合物,以及选自分子伴侣的肽基 - 脯氨酰基异构酶类的伴侣。 还描述了分别在HIV-1 gp41或HIV-2 gp36的N-螺旋结构域中包含特异性氨基酸取代的变体。
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70.发明授权Method for structuring a copper and/or permalloy layer by means of dry etching 失效通过干蚀刻来构造铜和/或坡莫合金层的方法
公开(公告)号:US4838994A
公开(公告)日:1989-06-13
申请号:US602307
申请日:1988-06-06
申请人: Peter Gulde , Christian Scholz
发明人: Peter Gulde , Christian Scholz
CPC分类号: G11B5/3163 , H01F41/34
摘要: A copper and/or permalloy layer is structured by means of dry etching. A layer of tantalum is applied as a mask to a layer to be structured, and a photoresist layer is applied to the tantalum layer. Subsequently, the structure of the photoresist layer generated in a photolithographic manner is transferred onto the mask by reactive ion etching. This procedure is continued until the copper or permalloy layer to be structured is exposed. The structuring of the copper or permalloy layer then occurs by ion beam etching.
摘要翻译: 通过干蚀刻来构造铜和/或坡莫合金层。 将一层钽作为掩模施加到待构造的层上,并且将光致抗蚀剂层施加到钽层。 随后,通过反应离子蚀刻将以光刻方式生成的光致抗蚀剂层的结构转移到掩模上。 继续该程序直到暴露出要结构的铜或坡莫合金层。 然后通过离子束蚀刻发生铜或坡莫合金层的构造。
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