Fan Xiang-xue, Tao Ran, Huang Jia-quan, Deng Ju-hong, Li Lan, Ma Ke, Xu Lei, Ning Qin
Zhongguo Ji Sheng Chong Xue Yu Ji Sheng Chong Bing Za Zhi. 2014 Aug;32(4):258-63.
To construct a short hairpin RNA (shRNA) against HSP47 gene, assess the expression level of HSP47 gene in NIH/3T3 cells, and observe the influence on cell function.
The HSP47-shRNA sequence presented at the downstream of the U6 promoter. The shRNA expression constructs were created using PCR- based methods. The PCR product was digested with Nhe I/Hind Ill and ligated into pGCsi/U6/Neo vector to produce HSP47-pGCsi-U6-shRNA (HSP47-1-pGCsi-U6-shRNA, HSP47-2-pGCsi-U6-shRNA and HSP47-3-pGCsi-U6-shRNA). The non-interference vector and non-related interference vector served as control. The vectors were transfected into NIH/3T3 fibroblast cells by liposome mediated gene transfection method. Transfection efficiency and fluorescence intensity were determined by fluorescence microscopy at 12, 24, 48, and 72 hours after transfection, respectively. Cells were collected before transfection, and at 24, and 48 hours post-transfection, respectively, HSP47 mRNA and protein expression levels were assessed by real-time PCR and Western blotting. The mRNA expression of TGF-pl, collagen types I and Ill in NIH/3T3 cells, and TGF-beta1 levels in cell culture supernatant were determined.
HSP47-shRNA vector was transfected into NIH/3T3 cells by liposome-mediated transfection. The transfection efficiency in each HSP47-shRNA plasmid interference group was about 60.0%, and there is no statistical difference among the interference groups (P> 0.05). A small amount of green fluorescent cells were found at 12 h post-transfection. The number of green fluorescent cells increased with the transfection time, and reached strongest at 72 h after transfection. shRNA interference significantly inhabited HSP47 expression in NIHI/3T3 cells. At 24 h after transfection with HSP47-1-shRNA, the inhibition effect was the strongest, and the relative silence efficiency of HSP47 mRNA was (25.83?1.79)%, lower than that of control group and non-related group (P<0.05). Collagen synthesis and secretion by NIH/3T3 cells reduced significantly at 24 and 48 hours post-transfection with HSP47-1-shRNA; and there was a significant difference between HSP47-1-shRNA intervention group and non-related controls. After transfection for 24 and 48 h, mRNA expression of collagen types I and IlI decreased to (56.52 +/- 1.64)% and (53.48 +/- 2.54)%, (54.17 +/- 2.63)% and (50.21 +/- 2.34)%, respectively, significantly lower than that of the control group and non-related group (P<0.05); however, no significant difference was found among the interference groups (P>0.05). In each HSP47-shRNA plasmid interference group, TGF-p1 mRNA expression was the lowest at 24 h post-transfection. The relative mRNA expression level was (63.23?2.18)%, (64.5+3.17)%, and (75.19 +/- 4.20)% in HSP47-1-shRNA, HSP47-2-shRNA, HSP47-3-shRNA groups (P>0.05), respectively, lower than that of the control group and non-related group (P<0.01). At 24 and 48 h post-transfection, TGF-P131 expression was the lowest at 24 h post-transfection, and the relative expression level in HSP47-1-shRNA, HSP47-2-shRNA, HSP47-3-shRNA groups was (51.79 +/- 3.12)%, (66.67 +/- 2.13)%, and (69.61 +/- 3.65)%, respectively. Compared with control group, the expression of TGF-beta1 in HSP47-1-shRNA and HSP47-2-shRNA2 groups was significant inhibited, but there was no significantly difference between control group and HSP47-3-shRNA group (P>0.05).
HSP47-shRNA. interference plasmid is constructed. HSP47-shRNA effectively inhibits protein expression of HSP47, and results in changes of cell function.
构建针对HSP47基因的短发夹RNA(shRNA),评估HSP47基因在NIH/3T3细胞中的表达水平,并观察其对细胞功能的影响。
HSP47-shRNA序列位于U6启动子下游。采用基于PCR的方法构建shRNA表达载体。PCR产物经Nhe I/Hind III酶切后连接到pGCsi/U6/Neo载体上,构建HSP47-pGCsi-U6-shRNA(HSP47-1-pGCsi-U6-shRNA、HSP47-2-pGCsi-U6-shRNA和HSP47-3-pGCsi-U6-shRNA)。以非干扰载体和非相关干扰载体作为对照。通过脂质体介导的基因转染方法将载体转染至NIH/3T3成纤维细胞。分别在转染后12、24、48和72小时通过荧光显微镜检测转染效率和荧光强度。在转染前、转染后24小时和48小时分别收集细胞,通过实时PCR和蛋白质印迹法评估HSP47 mRNA和蛋白表达水平。检测NIH/3T3细胞中TGF-β1、I型和III型胶原蛋白的mRNA表达以及细胞培养上清液中的TGF-β1水平。
通过脂质体介导的转染将HSP47-shRNA载体转染至NIH/3T3细胞。各HSP47-shRNA质粒干扰组的转染效率约为60.0%,各干扰组之间无统计学差异(P>0.05)。转染后12小时发现少量绿色荧光细胞。绿色荧光细胞数量随转染时间增加,在转染后72小时达到最强。shRNA干扰显著抑制了NIH/3T3细胞中HSP47的表达。转染HSP47-1-shRNA后24小时,抑制效果最强,HSP47 mRNA的相对沉默效率为(25.83±1.79)%,低于对照组和非相关组(P<0.05)。转染HSP47-1-shRNA后24小时和48小时,NIH/3T3细胞的胶原蛋白合成和分泌显著减少;HSP47-1-shRNA干预组与非相关对照组之间存在显著差异。转染24小时和48小时后,I型和III型胶原蛋白的mRNA表达分别降至(56.52±1.
