電轉化儀高效轉染mRNA進入小鼠受精卵形成穩定突變體
隨著小鼠基因組序列測序完成,許多研究都圍繞著功能基因參與的生物學過程,特別是發育和疾病研究領域。那么穩定遺傳修飾的模型動物對于闡明基因的作用十分重要,然而,傳統的方法,包括在胚胎干細胞中的同源重組或是構建小鼠嵌合體,既耗時又耗力。然而新的基因組編輯方法明顯的優化這個過程。在有效的基因組編輯方法中CRISPR/Cas 9系統是構建攜帶修飾基因組最簡單的方法。
雖然,CRISPR/Cas9系統簡化了形成突變體的過程,但是將DNAs/RNAs微注射入受精卵需要特殊的技術,得到大量的突變體也十分耗時間(注射數以百計的受精卵)。那么,為了簡化這個過程,我們嘗試用電轉化儀將RNA導入受精卵。
電轉也被用于過小鼠受精卵,但是過程涉及去除卵透明帶,或是用酸臺氏液薄化處理,這些對細胞是非常有毒性的,而且只有短小的RNAs(短于1kb)可以被導入。
近期,一只大鼠突變體成功構建,借助于在保持卵透明帶完好的前提下轉染Cas9mRNA和gRNA入大鼠受精卵。然而基因組編輯的效率很低(低于9%),而且需要大量的Cas9(1000-2000ng/ul)。
Figure 1. Optimal conditions for the electroporation used to deliver mRNA into fertilized eggs.(a) Electroporation set-up used in this study. The right box is the electroporator CUY21 EDIT II (BEX Co.Ltd),which generates electric pulsed, and the left is a stereoscopic microscope for embryo manipulation. Two electrodes were placed on the microscope stage and connected to the electroporator.
Figure 2. CRISPR/Cas9mediated genome editing by electroporation. (b)Examples of embryos from the three classes that exhibited different limb phenotypes: no limbs (type I), limb defects (type II, left hind limb deficiency, right: truncated fore-and hind-limb) , and normal (type III).(c)Graph summarizing the effects of Cas9 and gRNA electro-poration on limb development. The concentrations of RNAs used in each experiment are shown at left. The numbers in each column are the number of embryos exhibiting the phe-notype in each category.
Figure 3. The single-stranded oligodeoxynucleotide(ssODN)-induced generation of HDR-mediated instertions.(b) Representative embryo electroporated with Cas9 mRNA, gRNA, and ssODN.The mCherry florescene completely disappeared in the electroporated embryos, while control (no electroporation) embryos displayed florescent signals.
接下來,我們揭示了這種突變是否會在下一代中遺傳下來。電轉200ng/ul Cas9 mRNA和100ng/ul的gRNA入卵細胞,靶向mCherry基因。觀察25只F0代小鼠,均無紅色熒光表達。而且所有的F1代小鼠同樣沒有紅色熒光,而且mCherry基因被打斷。說明基因編輯突變體可以穩定遺傳。
討論
