• Asian-Australasian Journal of Animal Sciences
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• 제30권6호
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• pp.886-892
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• 2017

Objective: Transgenic technology is widely used for industrial applications and basic research. Systems that allow for genetic modification play a crucial role in biotechnology for a number of purposes, including the functional analysis of specific genes and the production of exogenous proteins. In this study, we examined and verified the cumate-inducible transgene expression system in chicken DF1 and quail QM7 cells, as well as loxP element-mediated transgene recombination using Cre recombinase in DF1 cells. Methods: After stable transfer of the transgene with piggyBac transposon and transposase, transgene expression was induced by an appropriate concentration of cumate. Additionally, we showed that the transgene can be replaced with additional transgenes by co-transfection with the Cre recombinase expression vector. Results: In the cumate-GFP DF1 and QM7 cells, green fluorescent protein (GFP) expression was repressed in the off state in the absence of cumate, and the GFP transgene expression was successfully induced in the presence of cumate. In the cumate-MyoD DF1 cells, MyoD transgene expression was induced by cumate, and the genes controlled by MyoD were upregulated according to the number of days in culture. Additionally, for the translocation experiments, a stable enhanced green fluorescent protein (eGFP)-expressing DF1 cell line transfected with the loxP66-eGFP-loxP71 vector was established, and DsRed-positive and eGFP-negative cells were observed after 14 days of co-transfection with the DsRed transgene and Cre recombinase indicating that the eGFP transgene was excised, and the DsRed transgene was replaced by Cre recombination. Conclusion: Transgene induction or replacement cassette systems in avian cells can be applied in functional genomics studies of specific genes and adapted further for efficient generation of transgenic poultry to modulate target gene expression.

• Journal of Microbiology and Biotechnology
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• 제24권4호
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• pp.568-576
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• 2014

TIM-1 (also known as KIM-1 and HAVcr-1) is a type I transmembrane glycoprotein member of the TIM family that may play important roles in innate and adaptive immune responses. The overexpression of proteins associated with membrane proteins is a major obstacle to overcome in studies of membrane protein structures and functions. In this study, we successfully coupled the overexpression of the TIM-1 protein with a C-terminal enhanced green fluorescent protein (GFP) tag in Escherichia coli. To the best of our knowledge, this report is the first to describe the overexpression of human TIM-1 in E. coli. The purified TIM-1-EGFP fusion protein recognized and bound directly to apoptotic cells and did not to bind to viable cells. Furthermore, we confirmed that the interactions of TIM-1-EGFP with apoptotic cells were blocked by TIM-1-Fc fusion proteins. This fusion protein represents a readily obtainable source of biologically active TIM-1 that may prove useful in future studies of human TIM-1.

• Journal of Microbiology and Biotechnology
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• 제22권9호
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• pp.1271-1278
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• 2012

Genetic fusion of two proteins frequently induces beneficial effects to the proteins, such as increased solubility, besides the combination of two protein functions. Here, we study the effects of the bacterial surface layer protein SgsE from Geobacillus stearothermophilus NRS 2004/3a on the folding of a C-terminally fused enhanced green fluorescent protein (EGFP) moiety. Although GFPs are generally unable to adopt a functional confirmation in the bacterial periplasm of Escherichia coli cells, we observed periplasmic fluorescence from a chimera of a 150-amino-acid N-terminal truncation of SgsE and EGFP. Based on this finding, unfolding and refolding kinetics of different S-layer-EGFP chimeras, a maltose binding protein-EGFP chimera, and sole EGFP were monitored using green fluorescence as indicator for the folded protein state. Calculated apparent rate constants for unfolding and refolding indicated different folding pathways for EGFP depending on the fusion partner used, and a clearly stabilizing effect was observed for the SgsE_C fusion moiety. Thermal stability, as determined by differential scanning calorimetry, and unfolding equilibria were found to be independent of the fused partner. We conclude that the stabilizing effect SgsE_C exerts on EGFP is due to a reduction of degrees of freedom for folding of EGFP in the fused state.

• Journal of Applied Biological Chemistry
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• 제66권
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• pp.128-137
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• 2023

Transcriptome analysis revealed that the sinR gene encoding a transition-state regulator of Bacillus pumilus, genetically close to B. subtilis, was expressed at high levels during growth. The sinR gene is the second gene of the sinIR operon consisting of three promoters and two structural genes in B. subtilis. This study used the sinIR promoter of B. subtilis DB104 to construct a recombinant protein expression system. First, the expression ability depending on the number of sinIR promoter was investigated using enhanced green fluorescent protein (eGFP). The expression level of eGFP was slightly higher when using two promoters (Psin2) than using original promoters. The Psin2 promoter was further engineered by modifying the repressor binding site and -35 and -10 regions. Shine-Dalgarno (SD) sequence of the sinI gene was modified to the consensus sequence. Finally, combining the engineered Psin2 promoter with the modified SD sequence increased the expression level of eGFP by about 13.4-fold over the original promoter. Our results suggest that the optimized sinIR promoter could be used as a novel tool for recombinant protein expression in B. subtilis.

• Clinical and Experimental Reproductive Medicine
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• 제36권4호
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• pp.283-292
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• 2009

목 적: 인간 배아줄기세포 (human embryonic stem cells; hESCs)는 체외에서 오랫동안 증식할 수 있으며, 모든 종류의 세포로 분화할 수 있는 능력을 가진 세포이다. 그러므로, 인간 배아줄기세포는 세포치료의 세포공급원의 역할을 할 수 있을 것으로 기대를 모으고 있다. 인간 배아줄기세포로의 외래 유전자의 도입은 분화경로 규명 및 특정 유전자의 기능 규명 등에 효과적으로 이용될 수 있다. 본 연구에서는 렌티 바이러스를 이용하여 eGFP 유전자를 XY와 XX 핵형을 가진 인간 배아줄기세포주에 도입하고자 하였다. 연구방법: 렌티 바이러스를 이용하여 eGFP 유전자를 인간 배아줄기세포에 도입하였다. 도입된 eGFP의 발현은 형광현미경을 이용하여 확인하였으며, 유세포 분석을 통하여 eGFP 발현세포의 비율을 분석하였다. 또한, eGFP가 도입된 인간 배아줄기세포에서 표지인자인 Oct4, SSEA4 및 Tra-1-81의 발현을 확인하였으며, 배아체의 형성 여부를 확인하여 특성분석을 수행하였다. 결 과: eGFP는 인간 배아줄기세포로 성공적으로 도입되었다. eGFP의 발현은 40 계대 이상 안정적으로 지속되었다. eGFP를 발현하는 인간 배아줄기세포는 eGFP 도입 후에도, 배아줄기세포의 특성을 유지하고 있음이 확인되었다. 또한, 자연적 분화 동안 발현이 감소하는 현상이 관찰되었다. 결 론: 본 연구에서는 렌티 바이러스를 이용하여 eGFP가 도입된 인간 배아줄기세포주를 확립하였으며, 그 특성이 유지되고 있음을 확인하였다. 표지 유전자가 도입된 인간 배아줄기세포주는 분화 및 다른 연구에 활용될 수 있을 것으로 기대된다.

• Clinical and Experimental Pediatrics
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• 제50권10호
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• pp.1011-1017
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• 2007

목 적 : 쥐의 섬유아세포인 NIH 3T3와 eGFP 유전자를 표지로 하는 레트로바이러스 벡터를 이용하여 유전자 전달효율을 향상시킬 수 있는 조건들을 살펴보고자 하였다. 방 법 : 표적세포에 대한 벡터의 비율과(1:1-1:8) 전달감염 횟수를 변화시켰을 때(1회, 2회), 양이온 복합체인 polybrene($4{\mu}g/mL$)을 첨가하였을 때 유전자 전달효율의 변화를 분석하였다. eGFP 유전자의 발현을 확인하기 위하여 형광 현미경 하에서 녹색빛을 내는 세포들을 관찰하고 FACscan으로 eGFP 양성세포의 비율을 측정하였다. 결 과 : 유전자 전달효율은 벡터와 표적세포의 비율 1:1에서 7%, 1:4에서 38%로 표적세포에 대한 레트로바이러스 벡터의 비율이 높을수록 상승하였지만 비율 1:4와 1:8사이에서는 차이가 없었다. 전달감염을 두 번 시행하는 것이 벡터와 표적세포의 비율 1:4까지는 유전자 전달효율에 영향을 미치지 않았지만 비율 1:8에서는 유전자 전달효율을 증가시켰다. 전달감염 후 eGFP 유전자의 발현은 3회 계대배양까지 약 3배 가량 증가하였지만 이후에는 감소하였는데 이와 같은 감소 정도는 전달감염을 한 번 시행한 경우가 두 번 시행한 경우보다 더 커서 전달감염을 반복하는 것이 유전자 전달효율의 증가효과보다는 주입된 유전자의 지속발현에 더 영향을 미치는 것으로 판단되었다. Polybrene을 첨가하였을 때 유전자 전달효율은 5.8%에서 38.8%로 대폭 상승하였으며 독성반응은 관찰되지 않았다. 배양접시의 크기에 따른 유전자 전달효율을 비교하였을 때 NIH 3T3세포의 증식정도는 6-well plate가 더 컸지만 eGFP 양성세포의 비율은 24-well plate에서 더 높았다. 결 론 : 이번 연구결과를 기초로 삼아 유전자 치료의 연구를 발전시키고 특히 전달된 유전자의 안정적인 발현과 바이러스 벡터들의 독성 등에 대하여 향후 연구의 초점을 두어야 할 것으로 생각된다.

• Maxillofacial Plastic and Reconstructive Surgery
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• 제28권5호
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• pp.375-395
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• 2006

Purpose: Lingual nerve (LN) damage may be caused by either tumor resection or injury such as wisdom tooth extraction, Although autologous nerve graft is sometimes used to repair the damaged nerve, it has the disadvantage of necessity of another operation for nerve harvesting. Moreover, the results of nerve grafting is not satisfactory. The nerve growth factor (NGF) is well-known to play a critical role in peripheral nerve regeneration and its local delivery to the injured nerve has been continuously tried to enhance nerve regeneration. However, its application has limitations like repeated administration due to short half life of 30 minutes and an in vivo delivery model must allow for direct and local delivery. The aim of this study was to construct a well-functioning $rhNGF-{\beta}$ adenovirus for the ultimate development of improved method to promote peripheral nerve regeneration with enhanced and extended secretion of hNGF from the injured nerve by injecting $rhNGF-{\beta}$ gene directly into crush-injured LN in rat model. Materials and Methods: $hNGF-{\beta}$ gene was prepared from fetal brain cDNA library and cloned into E1/E3 deleted adenoviral vector which contains green fluorescence protein (GFP) gene as a reporter. After large scale production and purification of $rhNGF-{\beta}$ adenovirus, transfection efficiency and its expression at various cells (primary cultured Schwann cells, HEK293 cells, Schwann cell lines, NIH3T3 and CRH cells) were evaluated by fluorescent microscopy, RT-PCR, ELISA, immunocytochemistry. Furthermore, the function of rhNGF-beta, which was secreted from various cells infected with $rhNGF-{\beta}$ adenovirus, was evaluated using neuritogenesis of PC-12 cells. For in vivo evaluation of efficacy of $rhNGF-{\beta}$ adenovirus, the LNs of 8-week old rats were exposed and crush-injured with a small hemostat for 10 seconds. After the injury, $rhNGF-{\beta}$ adenovirus($2{\mu}l,\;1.5{\times}10^{11}pfu$) or saline was administered into the crushed site in the experimental (n=24) and the control group (n=24), respectively. Sham operation of another group of rats (n=9) was performed without administration of either saline or adenovirus. The taste recovery and the change of fungiform papilla were studied at 1, 2, 3 and 4 weeks. Each of the 6 animals was tested with different solutions (0.1M NaCl, 0.1M sucrose, 0.01M QHCl, or 0.01M HCl) by two-bottle test paradigm and the number of papilla was counted using SEM picture of tongue dorsum. LN was explored at the same interval as taste study and evaluated electro-physiologically (peak voltage and nerve conduction velocity) and histomorphometrically (axon count, myelin thickness). Results: The recombinant adenovirus vector carrying $rhNGF-{\beta}$ was constructed and confirmed by restriction endonuclease analysis and DNA sequence analysis. GFP expression was observed in 90% of $rhNGF-{\beta}$ adenovirus infected cells compared with uninfected cells. Total mRNA isolated from $rhNGF-{\beta}$ adenovirus infected cells showed strong RT-PCR band, however uninfected or LacZ recombinant adenovirus infected cells did not. NGF quantification by ELISA showed a maximal release of $18865.4{\pm}310.9pg/ml$ NGF at the 4th day and stably continued till 14 days by $rhNGF-{\beta}$ adenovirus infected Schwann cells. PC-12 cells exposed to media with $rhNGF-{\beta}$ adenovirus infected Schwann cell revealed at the same level of neurite-extension as the commercial NGF did. $rhNGF-{\beta}$ adenovirus injected experimental groups in comparison to the control group exhibited different taste preference ratio. Salty, sweet and sour taste preference ratio were significantly different after 2 weeks from the beginning of the experiment, which were similar to the sham group, but not to the control group.