Computer Science and Artificial Intelligence Laboratory, Massachusetts Institute of Technology, Cambridge, MA 02139, USA.
J Biol Eng. 2010 Dec 20;4:17. doi: 10.1186/1754-1611-4-17.
BioBrick standard biological parts are designed to make biological systems easier to engineer (e.g. assemble, manipulate, and modify). There are over 5,000 parts available in the Registry of Standard Biological Parts that can be easily assembled into genetic circuits using a standard assembly technique. The standardization of the assembly technique has allowed for wide distribution to a large number of users -- the parts are reusable and interchangeable during the assembly process. The standard assembly process, however, has some limitations. In particular it does not allow for modification of already assembled biological circuits, addition of protein tags to pre-existing BioBrick parts, or addition of non-BioBrick parts to assemblies.
In this paper we describe a simple technique for rapid generation of synthetic biological circuits using introduction of customized inserts. We demonstrate its use in Escherichia coli (E. coli) to express green fluorescent protein (GFP) at pre-calculated relative levels and to add an N-terminal tag to GFP. The technique uses a new BioBrick part (called a BioScaffold) that can be inserted into cloning vectors and excised from them to leave a gap into which other DNA elements can be placed. The removal of the BioScaffold is performed by a Type IIB restriction enzyme (REase) that recognizes the BioScaffold but cuts into the surrounding sequences; therefore, the placement and removal of the BioScaffold allows the creation of seamless connections between arbitrary DNA sequences in cloning vectors. The BioScaffold contains a built-in red fluorescent protein (RFP) reporter; successful insertion of the BioScaffold is, thus, accompanied by gain of red fluorescence and its removal is manifested by disappearance of the red fluorescence.
The ability to perform targeted modifications of existing BioBrick circuits with BioScaffolds (1) simplifies and speeds up the iterative design-build-test process through direct reuse of existing circuits, (2) allows incorporation of sequences incompatible with BioBrick assembly into BioBrick circuits (3) removes scar sequences between standard biological parts, and (4) provides a route to adapt synthetic biology innovations to BioBrick assembly through the creation of new parts rather than new assembly standards or parts collections.
生物积木标准生物部件旨在使生物系统更容易进行工程设计(例如组装、操作和修改)。在标准生物部件注册中心有超过 5000 个部件可供使用,这些部件可以使用标准组装技术轻松组装成遗传电路。组装技术的标准化允许广泛分发给大量用户 - 部件在组装过程中是可重复使用和可互换的。然而,标准组装过程存在一些限制。特别是,它不允许修改已组装的生物电路,向现有的生物积木部件添加蛋白质标签,或向组装物添加非生物积木部件。
在本文中,我们描述了一种使用自定义插入物快速生成合成生物电路的简单技术。我们在大肠杆菌(E. coli)中证明了其用途,以预先计算的相对水平表达绿色荧光蛋白(GFP)并在 GFP 上添加 N 端标签。该技术使用一种新的生物积木部件(称为生物支架),可以插入克隆载体并从中切除,从而留下一个可以放置其他 DNA 元件的缺口。生物支架的去除是通过识别生物支架但切入周围序列的 IIB 型限制酶(REase)完成的;因此,生物支架的放置和去除允许在克隆载体中的任意 DNA 序列之间创建无缝连接。生物支架包含内置的红色荧光蛋白(RFP)报告基因;生物支架的成功插入因此伴随着红色荧光的获得,其去除表现为红色荧光的消失。
使用生物支架对现有生物积木电路进行靶向修饰的能力(1)通过直接重复使用现有电路简化和加快了迭代设计-构建-测试过程,(2)允许将与生物积木组装不兼容的序列纳入生物积木电路中,(3)去除标准生物部件之间的疤痕序列,(4)通过创建新部件而不是新的组装标准或部件集来为适应生物积木组装的合成生物学创新提供途径。
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