会员体验
专利管家(专利管理)
工作空间(专利管理)
风险监控(情报监控)
数据分析(专利分析)
侵权分析(诉讼无效)
联系我们
交流群
官方交流:
QQ群: 891211   
微信请扫码    >>>
现在联系顾问~
热词
    • 4. 发明申请
    • RNA ANALYTICS METHOD
    • RNA分析方法
    • WO2011070155A1
    • 2011-06-16
    • PCT/EP2010/069382
    • 2010-12-10
    • LEXOGEN GMBHSEITZ, AlexanderPAUL, LukasVAN MIN, Max Jan
    • SEITZ, AlexanderPAUL, LukasVAN MIN, Max Jan
    • C12Q1/68
    • C12Q1/6869C12Q1/6806C12Q1/6809C12Q2537/143C12Q2535/122C12Q2525/191C12Q2563/179C12Q2539/107
    • The present invention relates to a method of ordering nucleic acid molecule fragment sequences derived from a pool of potentially diverse RNA molecules comprising • optionally reverse transcribing the RNA molecules to provide a pool of cDNA molecules, • segregating nucleic acids from said template RNA or cDNA pool, selecting for potentially different templates with a distinctive nucleic acid feature shared by the segregated templates, thereby providing at least a first subpool of nucleic acids, • optionally once or more further segregating nucleic acids from said template RNA or cDNA, selectively segregating nucleic acids with a different distinctive nucleic acid feature, thereby providing one or more further subpool(s) of nucleic acids, • generating fragments of said segregated nucleic acid molecules by fragmenting or obtaining fragment copies of said segregated nucleic acid molecules, wherein the fragments of each subpool or combined subpools remain separable from fragments of other subpools or other combined subpools by physically separating the subpools or by attaching a label to the fragments of the subpools, with the label identifying a subpool, or determining a partial sequence of said segregated nucleic acid molecule and preferably aligning at least two sequences or partial sequences to a joined sequence.
    • 本发明涉及一种排序源自潜在不同RNA分子库的核酸分子片段序列的方法,其包括任选逆转录RNA分子以提供cDNA分子池,将核酸与所述模板RNA或cDNA库分离 选择具有由分离的模板共享的独特的核酸特征的潜在不同的模板,从而提供核酸的至少第一子池,任选地一次或多次将所述模板RNA或cDNA分离出来的核酸,选择性地将核酸与 不同的特征核酸特征,从而提供核酸的一个或多个另外的子区,通过片段化或获得所述分离的核酸分子的片段拷贝产生所述分离的核酸分子的片段,其中每个子池的片段或 组合子项目与ot的片段保持分离 她的子项目或其他组合子项目通过物理分离子项目或通过将标签附加到子项目的片段上,标签标识子项,或确定所述分离的核酸分子的部分序列,优选对齐至少两个序列或部分 序列到连接序列。
    • 5. 发明申请
    • METHOD AND MEANS FOR GENERATING TRANSCRIBED NUCLEIC ACIDS
    • WO2022069703A1
    • 2022-04-07
    • PCT/EP2021/077088
    • 2021-10-01
    • LEXOGEN GMBH
    • SURVILA, MantasMOLL, PamelaSEITZ, Alexander
    • C12Q1/6865C12Q2563/179
    • The present invention relates to a method of generating transcribed nucleic acids, comprising the steps of providing a nucleic acid template, hybridizing an oligonucleotide probe to the nucleic acid template, wherein said oligonucleotide probe comprises a complementary part that hybridizes to the nucleic acid template and a non-complementary part in (5') direction of the complementary part that does not hybridize to the nucleic acid template and comprises a sequence of a transcription promoter, hydrolysing a (3') part of the nucleic acid template that is in (3') direction to a part of the nucleic acid template that hybridizes to the oligonucleotide probe and wherein said (3') part is not hybridized to the oligonucleotide probe, or hydrolysing the nucleic acid template in the template-probe duplex to dissociate the (3') directed part of the template, extending the nucleic acid template with nucleic acids complementary to the non-complementary part of the oligonucleotide probe, thereby generating a duplex of the sequence of the transcription promoter in sequence with the nucleic acid template, transcribing the nucleic acid template with a transcriptase that binds the duplex of the sequence of the transcription promoter, thereby generating the transcribed nucleic acids; and kits and nucleic acids for performing such a method.
    • 6. 发明申请
    • 5´ PROTECTION DEPENDENT AMPLIFICATION
    • 5保护依赖放大
    • WO2014009413A2
    • 2014-01-16
    • PCT/EP2013/064582
    • 2013-07-10
    • LEXOGEN GMBH
    • SEITZ, AlexanderGABLER, IrmlindPAUL, Lukas
    • C12N15/1096C12P19/34C12Q1/6844C12Q1/6858C12Q2521/107
    • The present invention relates to methods for generating a labelled nucleic acid from an RNA comprising a 5' protecting group, said method comprises the steps of obtaining a mixture of template strands of nucleic acids, said mixture comprising said RNA and further potentially other nucleic acids without a 5' protecting group, annealing at least one oligonucleotide primer to the template strand of said RNA and potentially other nucleic acids, and template sequence dependent extending said primer, thereby obtaining a complementary nucleic acid strand annealed to its template strand, or providing the RNA in duplex with a complementary nucleic acid strand annealed to its template strand, and optionally modifying the extension product of said nucleic acids without 5' protecting group either on the 5' end of the template strand or on the 3' end of the complementary strand, or both, and labelling a complementary nucleic acid of a double stranded nucleic acid not modified, wherein therefore the labelled nucleic acid did have a 5' protecting group on the RNA template strand, said 5' protecting group being optionally removed after modification, and/or labelling a complementary nucleic acid of a double strand dependent on the presence of the 5' protecting group on the complementary nucleic acids template RNA strand by double strand dependent ligation, thereby specifically generating a labelled nucleic acid complementary to an RNA at least originally comprising a 5' protecting group.
    • 本发明涉及从包含5'保护基团的RNA产生标记的核酸的方法,所述方法包括以下步骤:获得核酸模板链的混合物,所述混合物包含所述RNA和另外潜在的其它核酸,而没有 5'保护基团,至少一个寡核苷酸引物退火至所述RNA的模板链和潜在的其它核酸,以及延伸所述引物的模板序列,从而获得退火至其模板链的互补核酸链,或提供RNA 与退火至其模板链的互补核酸链双链体,并任选地在模板链的5'末端或互补链的3'末端修饰所述核酸的延伸产物,而没有5'保护基, 或两者,并标记未被修饰的双链核酸的互补核酸,其中因此 标记的核酸在RNA模板链上确实具有5'保护基团,所述5'保护基团在修饰后任选地被除去,和/或根据5'保护基团的存在来标记双链的互补核酸 互补核酸模板RNA链通过双链依赖性连接,从而特异性产生与至少最初包含5'保护基的RNA互补的标记核酸。
    • 7. 发明申请
    • NUCLEIC ACID TRANSCRIPTION METHOD
    • 核酸转录法
    • WO2013038010A2
    • 2013-03-21
    • PCT/EP2012/068250
    • 2012-09-17
    • LEXOGEN GMBH
    • SEITZ, AlexanderMOLL, PamelaNAPORA, Magdalena Anna
    • C12Q1/68
    • C12N15/1096C12Q1/6816C12Q1/6853C12Q2521/107C12Q2525/113C12Q2533/107C12Q2521/501C12Q2525/161
    • The present invention relates to methods for generating an amplified nucleic acid portion of a template nucleic acid, comprising obtaining said template nucleic acid, annealing at least one oligonucleotide primer to said template nucleic acid, annealing at least one oligonucleotide stopper to said template nucleic acid, elongating the at least one oligonucleotide primer in a template specific manner until the elongating product nucleic acid reaches the position of an annealed oligonucleotide stopper, whereby the elongation reaction is stopped, wherein in said elongation reaction said oligonucleotide stopper is not elongated, and wherein the elongated product nucleic acid is ligated to the 3' end of said oligonucleotide stopper -said stopper may also be a primer itself and uses and kits for performing said method.
    • 本发明涉及产生模板核酸扩增核酸部分的方法,包括获得所述模板核酸,将至少一种寡核苷酸引物退火至所述模板核酸,将至少一种寡核苷酸终止物退火至所述模板核酸, 以模板特异性方式延伸所述至少一种寡核苷酸引物直到所述延伸产物核酸达到退火的寡核苷酸终止位置,由此停止所述延伸反应,其中在所述延伸反应中所述寡核苷酸终止子不伸长,并且其中所述细长 产物核酸连接到所述寡核苷酸塞子的3'末端 - 塞子塞也可以是引物本身,并且用于和执行所述方法的试剂盒。