南方医科大学学报
南方醫科大學學報
남방의과대학학보
JOURNAL OF SOUTHERN MEDICAL UNIVERSITY
2014年
1期
96-99
,共4页
赵英鹏%李立%马菁番%白建华%刘其雨
趙英鵬%李立%馬菁番%白建華%劉其雨
조영붕%리립%마정번%백건화%류기우
慢病毒载体%转染%肝脏
慢病毒載體%轉染%肝髒
만병독재체%전염%간장
lentiviral vector%transfection%liver
目的:研究慢病毒载体基因在肝脏内转染的有效途径。方法本实验根据大鼠消化系统解剖,设计利用经回盲部回结肠静脉穿刺置管至门静脉作为转染途径。通过观察对比尾静脉转染途径大鼠肝脏荧光蛋白表达、基因表达及转氨酶变化情况,探讨不同转染方法的有效性和安全性。结果门静脉转染组和尾静脉转染组大鼠均存活。转染后96 h慢病毒载体携带绿色荧光蛋白在门静脉转染组肝脏呈高表达,14 d后仍有持续表达;尾静脉转染组术后96 h荧光蛋白表达较门静脉组弱,14 d后几无持续表达。RT-PCR检测转染基因LXRα-RNAi效率:转染组LXRαmRNA表达均有下调,门静脉转染组LXRα基因敲减率明显高于尾静脉转染组(0.135±0.002 vs 0.713±0.036,P<0.05),两组血清ALT比较差别无统计学意义。结论经门静脉灌注是基因转染的有效途径,经回盲部回结肠静脉属支穿刺置管可在保证大鼠存活的情况下提高基因转染率,且对肝功能无明显损害,是值得推广的方法。
目的:研究慢病毒載體基因在肝髒內轉染的有效途徑。方法本實驗根據大鼠消化繫統解剖,設計利用經迴盲部迴結腸靜脈穿刺置管至門靜脈作為轉染途徑。通過觀察對比尾靜脈轉染途徑大鼠肝髒熒光蛋白錶達、基因錶達及轉氨酶變化情況,探討不同轉染方法的有效性和安全性。結果門靜脈轉染組和尾靜脈轉染組大鼠均存活。轉染後96 h慢病毒載體攜帶綠色熒光蛋白在門靜脈轉染組肝髒呈高錶達,14 d後仍有持續錶達;尾靜脈轉染組術後96 h熒光蛋白錶達較門靜脈組弱,14 d後幾無持續錶達。RT-PCR檢測轉染基因LXRα-RNAi效率:轉染組LXRαmRNA錶達均有下調,門靜脈轉染組LXRα基因敲減率明顯高于尾靜脈轉染組(0.135±0.002 vs 0.713±0.036,P<0.05),兩組血清ALT比較差彆無統計學意義。結論經門靜脈灌註是基因轉染的有效途徑,經迴盲部迴結腸靜脈屬支穿刺置管可在保證大鼠存活的情況下提高基因轉染率,且對肝功能無明顯損害,是值得推廣的方法。
목적:연구만병독재체기인재간장내전염적유효도경。방법본실험근거대서소화계통해부,설계이용경회맹부회결장정맥천자치관지문정맥작위전염도경。통과관찰대비미정맥전염도경대서간장형광단백표체、기인표체급전안매변화정황,탐토불동전염방법적유효성화안전성。결과문정맥전염조화미정맥전염조대서균존활。전염후96 h만병독재체휴대록색형광단백재문정맥전염조간장정고표체,14 d후잉유지속표체;미정맥전염조술후96 h형광단백표체교문정맥조약,14 d후궤무지속표체。RT-PCR검측전염기인LXRα-RNAi효솔:전염조LXRαmRNA표체균유하조,문정맥전염조LXRα기인고감솔명현고우미정맥전염조(0.135±0.002 vs 0.713±0.036,P<0.05),량조혈청ALT비교차별무통계학의의。결론경문정맥관주시기인전염적유효도경,경회맹부회결장정맥속지천자치관가재보증대서존활적정황하제고기인전염솔,차대간공능무명현손해,시치득추엄적방법。
Objective To investigate the optimal approach of lentiviral vector transfection for effective delivery of exogenous gene into the liver. Methods The lentiviral vector was delivered via the ileocolic vein of the ileocecus (portal vein group) or via the caudal vein of SD rats. The effect gene transfection into the liver was assessed by observing the expression of green fluorescence protein expression carried by the lentiviral vector, silencing of LXRα mRNA expression mediated by RNA interference, and liver transaminase changes. The efficiency and safety of the two approaches of transfection were evaluated. Results All the rats receiving lentiviral transfection survived. In the portal vein group, abundant green fluorescence was detected in the liver at 96 h following the trasnfection and lasted till 14 days, whereas only weak fluorescence was observed in the caudal vein group. The results of RT-PCR demonstrated a significant higher rate of LXRαknock-down in portal vein group than in caudal vein group (0.135 ± 0.002 vs 0.713 ± 0.036, P<0.05). No significant difference in ALT levels found between the two groups. Conclusion Infusion via the potal vein is effective for gene transfection into the liver, and puncture from the ileocolic vein of ileocecus can guarantee the survival of rats and improve the transfection efficiency without causing liver injury.
