- 作者:Yajing Wang ; Shuhuan Shang ; shuhuans@aliyun.com" class="auth_mail" title="E-mail the corresponding author ; Chengzhang Li ; lcz56@163.com" class="auth_mail" title="E-mail the corresponding author
- 关键词:human periodontal ligament stem cells ; nonviral vectors ; transfection efficiency
- 刊名:Journal of Dental Sciences
- 出版年:2015
- 出版时间:December 2015
- 年:2015
- 卷:10
- 期:4
- 页码:414-422
- 全文大小:3060 K
Materials and methods
The hPDLSCs were transfected by (1) Lipofectamine 2000, (2) polyethylenimine, (3) GBfectene-Elite transfection reagent, (4) X-tremeGENE HP DNA Transfection Reagent, and (5) Magnet-Assisted Transfection (MATra), compared to (6) lentiviral vectors harboring a green-fluorescent-protein gene. The transfection efficiency was measured by a fluorescence microscope and flow cytometry. Meanwhile, the cell morphology and growth status were observed to estimate the cytotoxicity.
Results
Among these methods, the transfection efficiency of the former four methods was not very satisfactory (< 6%) compared to that of lentiviral vectors (positive control, 95%). However, MATra was the most effective nonviral method (11%). Moreover, the cellular toxicity was lower than that of the former four methods.
Conclusion
The transfection efficiency of hPDLSCs with MATra was higher than the other nonviral transfection reagents in this study, but it was far less than the viral vectors. Saving from the interaction between the positive and negative charges, and increasing the opportunity of contact between the plasmid and the cytomembrane might be the key to enhancing the transfection efficiency for hPDLSCs in application of periodontal tissue engineering.