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使用纤维修饰腺病毒载体对培养中的分散胰岛细胞进行高效基因转导

Efficient Gene Transduction of Dispersed Islet Cells in Culture Using Fiber-Modified Adenoviral Vectors.

作者信息

Hanayama Hiroyuki, Ohashi Kazuo, Utoh Rie, Shimizu Hirofumi, Ise Kazuya, Sakurai Fuminori, Mizuguchi Hiroyuki, Tsuchiya Hiroyuki, Okano Teruo, Gotoh Mitsukazu

机构信息

Department of Regenerative Surgery, Fukushima Medical University , Hikarigaoka, Fukushima , Japan.

† iPS Cell-based Projects on Cell Transplantation and Cell Dynamics, Graduate School of Pharmaceutical Sciences, Osaka University , Suita, Osaka , Japan.

出版信息

Cell Med. 2015 Aug 26;8(1-2):31-8. doi: 10.3727/215517915X689083. eCollection 2015 Dec 17.

Abstract

To establish novel islet-based therapies, our group has recently developed technologies for creating functional neo-islet tissues in the subcutaneous space by transplanting monolithic sheets of dispersed islet cells (islet cell sheets). Improving cellular function and viability are the next important challenges for enhancing the therapeutic effects. This article describes the adenoviral vector-mediated gene transduction of dispersed islet cells under culture conditions. Purified pancreatic islets were obtained from Lewis rats and dissociated into single islet cells. Cells were plated onto laminin-5-coated temperature-responsive polymer poly(N-isopropylacrylamide)-immobilized plastic dishes. At 0 h, islet cells were infected for 1 h with either conventional type 5 adenoviral vector (Ad-CA-GFP) or fiber-modified adenoviral vector (AdK7-CA-GFP) harboring a polylysine (K7) peptide in the C terminus of the fiber knob. We investigated gene transduction efficiency at 48 h after infection and found that AdK7-CA-GFP yielded higher transduction efficiencies than Ad-CA-GFP at a multiplicity of infection (MOI) of 5 and 10. For AdK7-CA-GFP at MOI = 10, 84.4 ± 1.5% of islet cells were found to be genetically transduced without marked vector infection-related cellular damage as determined by viable cell number and lactate dehydrogenase (LDH) release assay. After AdK7-CA-GFP infection at MOI = 10, cells remained attached and expanded to nearly full confluency, showing that this adenoviral infection protocol is a feasible approach for creating islet cell sheets. We have shown that dispersed and cultured islet cells can be genetically modified efficiently using fiber-modified adenoviral vectors. Therefore, this gene therapy technique could be used for cellular modification or biological assessment of dispersed islet cells.

摘要

为了建立新的基于胰岛的治疗方法,我们团队最近开发了通过移植分散胰岛细胞的整体片层(胰岛细胞片层)在皮下空间创建功能性新胰岛组织的技术。改善细胞功能和活力是增强治疗效果的下一个重要挑战。本文描述了在培养条件下腺病毒载体介导的分散胰岛细胞的基因转导。从Lewis大鼠中获得纯化的胰岛,并将其解离为单个胰岛细胞。将细胞接种到包被层粘连蛋白-5的温度响应性聚合物聚(N-异丙基丙烯酰胺)固定化塑料培养皿上。在0小时时,胰岛细胞用传统的5型腺病毒载体(Ad-CA-GFP)或在纤维旋钮C末端含有聚赖氨酸(K7)肽的纤维修饰腺病毒载体(AdK7-CA-GFP)感染1小时。我们在感染后48小时研究了基因转导效率,发现AdK7-CA-GFP在感染复数(MOI)为5和10时比Ad-CA-GFP产生更高的转导效率。对于MOI = 10的AdK7-CA-GFP,通过活细胞数和乳酸脱氢酶(LDH)释放试验确定,发现84.4±1.5%的胰岛细胞被基因转导,且无明显的载体感染相关细胞损伤。在MOI = 10的AdK7-CA-GFP感染后,细胞保持附着并扩展至几乎完全汇合,表明这种腺病毒感染方案是创建胰岛细胞片层的可行方法。我们已经表明,使用纤维修饰的腺病毒载体可以有效地对分散和培养的胰岛细胞进行基因改造。因此,这种基因治疗技术可用于分散胰岛细胞的细胞修饰或生物学评估。

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本文引用的文献

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Quality of Air-Transported Human Islets for Single Islet Cell Preparations.用于单个胰岛细胞制备的空运人胰岛的质量
Cell Med. 2013 Oct 23;6(1-2):33-8. doi: 10.3727/215517913X674243. eCollection 2013 Dec 30.
3
Current status of clinical islet transplantation.临床胰岛移植的现状
World J Transplant. 2013 Dec 24;3(4):48-53. doi: 10.5500/wjt.v3.i4.48.
4
Functional tissue engineering of the liver and islets.肝脏和胰岛的功能性组织工程。
Anat Rec (Hoboken). 2014 Jan;297(1):73-82. doi: 10.1002/ar.22810. Epub 2013 Dec 2.
7
Biosafety features of lentiviral vectors.慢病毒载体的生物安全性特征。
Hum Gene Ther. 2013 Feb;24(2):132-42. doi: 10.1089/hum.2012.229.

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