公开(公告)号：US4999293A

公开(公告)日：1991-03-12

申请号：US134237

申请日：1987-12-17

申请人： Janet M. Barsomian ,  Geoffrey G. Wilson

发明人： Janet M. Barsomian ,  Geoffrey G. Wilson

IPC分类号： C12N9/12 ,  C12N1/20 ,  C12N9/10 ,  C12N9/16 ,  C12N9/22 ,  C12N15/09 ,  C12R1/19 ,  C12R1/21

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： The present invention is directed to a method for cloning and producing the HhaI restriction endonuclease by (1) introducing the restriction endonuclease gene from Haemophilus haemolyticus ATCC 10014 into a host whereby the restriction gene is expressed; (2) fermenting the host which contains the vector encoding and expressing the HhaI restriction endonuclease, and (3) purifying the HhaI restriction endonuclease from the fermented host which contains the vector encoding and expressing the HhaI restriction endonuclease activity.

公开(公告)号：US4983522A

公开(公告)日：1991-01-08

申请号：US134235

申请日：1987-12-17

申请人： Janet M. Barsomian ,  Geoffrey G. Wilson

发明人： Janet M. Barsomian ,  Geoffrey G. Wilson

IPC分类号： C12N1/20 ,  C12N1/21 ,  C12N9/10 ,  C12N9/16 ,  C12N9/22 ,  C12N15/00 ,  C12N15/09 ,  C12R1/19 ,  C12R1/21

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： The present invention is directed to a method for cloning and producing the HinPI restriction endonuclease by (1) introducing the restriction endonuclease gene from Haemophilus influenza P1 into a host whereby the restriction gene is expressed; (2) fermenting the host which contains the vector encoding and expressing the HinPI restriction endonuclease, and (3) purifying the HinPI restriction endonuclease from the fermented host which contains the vector encoding and expressing the HinPI restriction endonuclease activity.

公开(公告)号：US06403354B1

公开(公告)日：2002-06-11

申请号：US09766055

申请日：2001-01-19

申请人： Shuang-yong Xu ,  James Samuelson ,  John Pelletier ,  Marion Sibley ,  Geoffrey G. Wilson

发明人： Shuang-yong Xu ,  James Samuelson ,  John Pelletier ,  Marion Sibley ,  Geoffrey G. Wilson

IPC分类号： C12N922

CPC分类号： C12N9/22 ,  C12N9/1007

摘要： The present invention relates to recombinant DNA which encodes the BstYI restriction endonuclease as well as BstYI methyltransferase, expression of BstYI restriction endonuclease and M.BstYI in E. coli cells containing the recombinant DNA. It also relates to methods for purification of the recombinant BstYI restriction endonuclease and BstYI methyltransferase.

摘要翻译： 本发明涉及编码BstYI限制性内切核酸酶以及BstYI甲基转移酶，BstYI限制性内切核酸酶和M.BstYI在含有重组DNA的大肠杆菌细胞中的表达的重组DNA。 它还涉及重组BstYI限制性内切核酸酶和BstYI甲基转移酶的纯化方法。

公开(公告)号：US5366882A

公开(公告)日：1994-11-22

申请号：US169950

申请日：1993-12-17

申请人： Keith D. Lunnen ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Geoffrey G. Wilson

IPC分类号： C12N9/10 ,  C12N9/22 ,  C12N15/53 ,  C12N15/70

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： In accordance with the present invention there is provided an isolated DNA coding for the Bg/I restriction endonuclease and modification methylase derived from Bacillus globigii RUB561 stain, as well as related methods for cloning said recombinant DNA. The present invention also relates to clones which express recombinant Bg/I restriction endonuclease and recombinant modification methylase produced from Bg/I recombinant DNA and to methods for producing said enzymes.

摘要翻译： 根据本发明，提供了编码Bg / I限制性内切核酸酶和衍生自芽孢杆菌RUB561染色体的修饰甲基化酶的分离的DNA，以及用于克隆所述重组DNA的相关方法。 本发明还涉及表达重组Bg / I限制性内切核酸酶和由Bg / I重组DNA产生的重组修饰甲基化酶的克隆和用于产生所述酶的方法。

公开(公告)号：US06210945B1

公开(公告)日：2001-04-03

申请号：US09587066

申请日：2000-06-02

申请人： Keith D. Lunnen ,  Richard D. Morgan ,  Timothy Meixsell ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Richard D. Morgan ,  Timothy Meixsell ,  Geoffrey G. Wilson

IPC分类号： C12N922

CPC分类号： C12N9/22

摘要： RsaI, a restriction enzyme from the bacterium Rhodopseudomonas sphaeroides, recognizes the DNA sequence 5′-GTAC-3′. Because RsaI is commercially valuable, we sought to overproduce it by cloning the genes for RsaI and its accompanying, modification, enzyme. The ‘methylase-selection’ method, the customary procedure for cloning restriction and modification genes, was applied to RsaI. The method yielded clones containing the methylase gene (rsaIM), but none containing both the methylase gene and the restriction gene (rsaIR). Inverse-PCR was then used to recover sections of the DNA downstream of rsaIM. These sections were sequenced, and the sequences were joined in silico to reveal the gene organization of the RsaI R-M system. By comparing the coding potential of the DNA with the N-terminal amino acid sequence of the purified RsaI restriction enzyme, we discovered that the RsaI R and M genes, rather than being adjacent-the situation that pertains in most R-M systems-are separated by an intervening gene of unknown function. Based on this information, the rsaIR gene was cloned by PCR instead of methylase-selection. These new clones proved to be highly unstable, however, even in the presence of the rsaIM gene. Various attempts were made to stabilize the gene, but most met with failure. Stability was finally achieved by introducing a second methylase gene, mjaVM, to augment the protection provided by rsaIM, and by tightly controlling the expression of rsaIR using a special two-promoter, anti-sense transcription, expression vector.

摘要翻译： 来自细菌Rhodopseudomonas sphaeroides的限制酶RsaI识别DNA序列5'-GTAC-3'。 由于RsaI具有商业价值，我们试图通过克隆RsaI及其伴随的修饰酶的基因来过度生产。 将“甲基化酶选择”方法，克隆限制和修饰基因的常规方法应用于RsaI，该方法产生含有甲基化酶基因（rsaIM）的克隆，但不含有甲基化酶基因和限制性基因（rsaIR）。 然后使用反向PCR来回收rsaIM下游DNA的切片，对这些切片进行测序，并将序列与硅胶连接以揭示RsaI RM系统的基因组织，通过将DNA的编码潜力与N 纯化的RsaI限制酶的末端氨基酸序列，我们发现RsaI R和M基因而不是与大多数RM系统相关的情况相邻 - 由未知功能的介入基因分离，基于该信息 ，通过PCR克隆rsaIR基因而不是甲基化酶选择，这些新克隆被证明是高度不稳定的，然而，即使在rsaIM基因的存在下，也进行了各种尝试 lize基因，但大多数遇到失败。 通过引入第二个甲基化酶基因mjaVM来增加rsaIM提供的保护，并通过使用特异的双启动子，反义转录，表达载体来严格控制rsaIR的表达，最终达到稳定性。

公开(公告)号：US5002882A

公开(公告)日：1991-03-26

申请号：US344268

申请日：1989-04-27

申请人： Keith D. Lunnen ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Geoffrey G. Wilson

IPC分类号： C12N1/21 ,  C12N9/10 ,  C12N9/16 ,  C12N9/22 ,  C12N15/09 ,  C12N15/54 ,  C12N15/55 ,  C12R1/19 ,  C12R1/64

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： The present invention is directed to a method for cloning and producing the XmaI restriction endonuclease by (1) introducing the restriction endonuclease gene from X. malvacaerum into a host whereby the restriction gene is expressed; (2) fermenting the host which contains the plasmid encoding and expressing the XmaI restriction endonuclease activity, and (3) purifying the XmaI restriction endonuclease from the fermented host which contains the plasmid encoding and expressing the XmaI restriction endonuclease activity.

公开(公告)号：US4987074A

公开(公告)日：1991-01-22

申请号：US134001

申请日：1987-12-17

申请人： Keith D. Lunnen ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Geoffrey G. Wilson

IPC分类号： C12N1/20 ,  C12N1/21 ,  C12N9/10 ,  C12N9/16 ,  C12N9/22 ,  C12N15/09 ,  C12R1/01 ,  C12R1/19

CPC分类号： C12N9/22 ,  C12N9/1007

摘要： The present invention is directed to a method for cloning and producing the HgiAI restriction endonuclease by (1) introducing the restriction endonuclease gene from Herpetosiphon giganteus into a host whereby the restriction gene is expressed; (2) fermenting the host which contains the vector encoding and expressing the HgiAI restriction endonuclease, and (3) purifying the HgiAI restriction endonuclease from the fermented host which contains the vector encoding and expressing the HgiAI restriction endonuclease activity.

公开(公告)号：US06958230B2

公开(公告)日：2005-10-25

申请号：US10668047

申请日：2003-09-22

申请人： Keith D. Lunnen ,  Theodore Davis ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Theodore Davis ,  Geoffrey G. Wilson

IPC分类号： C12N1/21 ,  C12N9/10 ,  C12N9/22 ,  C12N15/55

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： The present invention relates to: recombinant DNA encoding the SbfI restriction endonuclease as well as the SbfI methylase, and expression of the SbfI restriction endonuclease and SbfI methylase in E. coli cells containing the recombinant DNA; and methods for cloning the SbfI restriction gene (sbfIR) from Streptomyces species Bf-61 into E. coli by PCR. The method relied on primers based on DNA sequences predicted from amino acid sequences of the purified SbfI restriction endonuclease.

摘要翻译： 本发明涉及编码SbfI限制性内切核酸酶以及SbfI甲基化酶的重组DNA，以及含有重组DNA的大肠杆菌细胞中SbfI限制性内切核酸酶和SbfI甲基化酶的表达。 以及通过PCR将来自Streptomyces物种Bf-61的SbfI限制性基因（sbfIR）克隆到大肠杆菌中的方法。 该方法依赖于基于纯化的SbfI限制性内切核酸酶的氨基酸序列预测的DNA序列的引物。

公开(公告)号：US5030569A

公开(公告)日：1991-07-09

申请号：US440438

申请日：1989-11-20

申请人： Keith D. Lunnen ,  Geoffrey G. Wilson

发明人： Keith D. Lunnen ,  Geoffrey G. Wilson

IPC分类号： C12N1/21 ,  C12N9/10 ,  C12N9/22

CPC分类号： C12N9/22 ,  C12N9/1007

摘要： The present invention is directed to a method for cloning and producing the Afl II restriction endonuclease by 1) introducing the restriction endonuclease gene from Anabaena flos-aquae into a host whereby the restriction gene is expressed; 2) fermenting the host which contains the plasmid encoding and expressing the Afl II restriction endonuclease activity, and 3) purifying the Afl II restriction endonuclease from the fermented host which contains the plasmid encoding and expressing the Afl II restriction endonuclease activity.

摘要翻译： 本发明涉及一种用于克隆和产生AflⅡ限制性内切核酸酶的方法，其方法是1）将来自鱼腥藻的限制性内切核酸酶基因导入宿主，由此限制性基因被表达; 2）发酵含有编码并表达Af1Ⅱ限制性内切核酸酶活性的质粒的宿主，和3）从含有编码和表达AflⅡ限制性内切核酸酶活性的质粒的发酵宿主中纯化AflⅡ限制性内切核酸酶。

公开(公告)号：US5004691A

公开(公告)日：1991-04-02

申请号：US133957

申请日：1987-12-17

申请人： Shu-zi Chen ,  Geoffrey G. Wilson

发明人： Shu-zi Chen ,  Geoffrey G. Wilson

IPC分类号： C12N9/16 ,  C12N1/20 ,  C12N1/21 ,  C12N9/10 ,  C12N9/22 ,  C12N15/09 ,  C12R1/01 ,  C12R1/19

CPC分类号： C12N9/1007 ,  C12N9/22

摘要： The present invention is directd to a method for cloning and producing the AccI restriction endonuclease by (1) introducing the restriction endonuclease gene from into a host whereby the restriction gene is expressed; (2) fermenting the host which contains the plasmid encoding and expressing the AccI restriction endonuclease activity, and (3) purifying the AccI restriction endonuclease from the fermented host which contains the plasmid encoding and expressing the AccI restriction endonuclease activity.