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Serum-free transfection of CHO-cells with tailor-made unilamellar vesicles

机译:量身定制的单层囊泡无血清转染CHO细胞

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摘要

At present, a number of transfection techniques are available to introduce foreign DNA into cells, but still minimal intrusion or interference with normal cell physiology, low toxicity, reproducibility, cost efficiency and successful creation of stable transfectants are highly desirable properties for improved transfection techniques.For all previous transfection experiments done in our labs, using serum-free cultivated host cell lines, an efficiency value of ~0.1% for selection of stable cell lines has not been exceeded, consequently we developed and improved a transfection system based on defined liposomes, so-called large unilamellar vesicles, consisting of different lipid compositions to facilitate clone selection and increase the probability for creation of recombinant high-production clones. DNA and DOTAP/DOPE or CHEMS/DOPE interact by electrostatic means forming so-called lipoplexes (Even-Chen and Barenholz 2000) and the lipofection efficiency of those lipoplexes has been determined via confocal microscopy.In addition, the expression of the EGFP was determined by FACS to investigate transient as well as stable transfection and the transfection efficiency of a selection of different commercially available transfection reagents and kits has been compared to our tailor-made liposomes.
机译:目前,有许多转染技术可用于将外源DNA引入细胞,但是对于正常的细胞生理,低毒性,可再现性,成本效率以及成功创建稳定的转染子仍然是最小的侵入或干扰,这是改进转染技术的高度期望的特性。在我们实验室进行的所有先前转染实验中,使用无血清培养的宿主细胞系,选择稳定细胞系的效率值均未超过〜0.1%,因此,我们开发并改进了基于定义脂质体的转染系统,所谓的大单层囊泡,由不同的脂质成分组成,以促进克隆选择并增加产生重组高产克隆的可能性。 DNA和DOTAP / DOPE或CHEMS / DOPE通过静电作用相互作用形成所谓的脂质复合物(Even-Chen和Barenholz 2000),并通过共聚焦显微镜确定了这些脂质复合物的脂质转染效率,此外还确定了EGFP的表达通过FACS进行瞬时和稳定转染研究,并将选择的各种市售转染试剂和试剂盒的转染效率与我们量身定制的脂质体进行了比较。

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