• Molecules and Cells
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• 제27권5호
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• pp.583-589
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• 2009

GTP cyclohydrolase I (GTPCH) is a key enzyme in the de novo synthesis of tetrahydrobiopterin. Previously, the Drosophila melanogaster GTPCH gene has been shown to be expressed from two different promoters (P1 and P2). In our study, the 5'-flanking DNA regions required for P1 and P2 promoter activities were characterized using transient expression assay. The DNA regions between -98 and +31, and between -73 and +35 are required for efficient P1 and P2 promoter activities, respectively. The regions between -98 and -56 and between -73 and -41 may contain critical elements required for the expression of GTPCH in Drosophila. By aligning the nucleotide sequences in the P1 and P2 promoter regions of the Drosophila melanogaster and Drosophila virilrs GTPCH genes, several conserved elements including palindromic sequences in the regions critical for P1 and P2 promoter activities were identified. Western blot analysis of transgenic flies transformed using P1 or P2 promoter-lacZ fusion plasmids further revealed that P1 promoter expression is restricted to the late pupae and adult developmental stages but that the P2 promoter driven expression of GTPCH is constitutive throughout fly development. In addition, X-gal staining of the embryos and imaginal discs of transgenic flies suggests that the P2 promoter is active from stage 13 of embryo and is generally active in most regions of the imaginal discs at the larval stages.

• Asian-Australasian Journal of Animal Sciences
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• 제12권4호
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• pp.520-524
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• 1999

The present experiments were designed to examine whether exogenous DNA injected into the germinal crescent region (GCR) of early stage of developing embryos, which is considered to be the main place from which PGCs originate, can be transferred to recipient chicken embryos. In this experiment, Miw Z (DNA) dissolved in the transfection reagent (TR: Boehringer, Germany) was introduced into the GCR of donor embryos at stage 3-5 or 9-11, followed by continued incubation until the stage 13-15 of embryonic development. The PGCs collected from the embryonic blood vessels were examined for the incorporation of the injected DNA into the PGCs by the methods of X-gal staining and PCR analysis. As the results, the foreign DNA was successfully incorporated into the PGCS, leading to their transfer to the gonadal tissues. The present results, therefore, suggest that the early stage (3-5 or 9-11) of chicken embryonic development would be more successful than stage 13-15 in transferring exogenous genes to the recipient embryos, leading to the possibility of producing transgenic chicken medianting the PGCS.

• Asian-Australasian Journal of Animal Sciences
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• 제11권5호
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• pp.498-502
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• 1998

The present study was designed, fIrst to develop the new methodology to measure the bioluminescence activity easily in live developing bovine embryos by photoncounting, and secondly to compare the expression efficiency of four luciferase reporter genes in bovine embryos at four- to 16-cell stages. In experiment 1, equimolar pSVlacZ and pSVEluc were microinjected into the pronucleus of fertilized bovine oocytes. At 2 days after micro injection, bioluminescence activity of these embryos was measured by photoncounting with a luminometer for 1 min, and lacZ gene expression in the same embryos was assayed by X-gal staining. All the luciferase-positive oocytes showed some bacterial ${\beta}$-galactosidase activity irrespective of the intensity. In experiment 2, four firefly luciferase genes (pTKEluc, pTK6WEluc, pSVEluc and pMiwluc) were introduced by micro injection, and the injected embryos were cultured for the following 2 days. Detection of the luciferase gene expression was done by photoncounting at 5 to 55 min. Over the measurement period, the luciferase activity was almost constant irrespective of the transgenes microinjected. The luciferase activity and expression efficiency at 2 days after microinjection were not significantly affected by the difference in the microinjected transgenes. The present results demonstrated that the bioluminescence activity in live developing bovine embryos could be measured quickly by photoncounting.

• 한국동물학회지
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• 제38권2호
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• pp.196-203
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• 1995

The c-myc proto-oncogene, one of the immediately earlY genes, is expressed in various mammalian cell types and heavily involved in the regulation of cell proliferation and differentiation. To determine endogeneous expression pattern of c-myc gene in preimpBantation mouse embwos, we employed a reverse transcription coupled to polvrnerase chain reaction (RT-PCR). Transcript of c-myc was detected at fertilized embryos as a maternal transcript. At the early two-cell stave, transcript of c-myc gene was hardly detected, bu, appeared at late two-cell embryos as a zygotic transcript. The level of c-myc expresion was increased at later stases and peaked at blastocvst stage. To examine the functional role of promoter region for c-myc gene transcription, we fused the 5'upstream region (1.8 kb) including econ 1 of c-myc genomic DNA with E. coli lacE gene fnamed as pcMYC-laczl. pcMYC-lacZ was microiniected into the pronscleus of mouse one-cell embryovs, and p·salactosidase activity was determined tv histochemical staining with X-gal at different stases. f-galactosidase activity was detected only at blastocyst, but not at the earlier stage embryos. This result indicates that c-myc gene is transcriptionallv active during mouse preimplantation development.

• Journal of Chest Surgery
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• 제41권5호
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• pp.550-562
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• 2008

배경: 조직공학분야에서 이종조직의 세포성분에 대한 면역반응을 없애기 위한 기본적인 과정으로 조직의 탈세포화에 대한 연구가 있어왔다. 본 연구는 기존에 탈세포화에 효과적이었다고 보고되었던 방법들을 변형 혹은 재현해 보고, 이를 통해 치적의 탈세포화를 얻을 수 있는 조건을 찾고자 하였다. 대상 및 방법: 돼지의 대동맥 및 폐동맥판막, 대동맥 및 폐동맥벽, 심낭을 탈세포화 세정제(detergents)에 대한 농도 및 배양시간, 온도조건, 용질에 대한 삼투압 등을 달리하고, 여러 탈세포화용액 및 그 조합을 통해 단일단계 및 여러 단계의 방법으로 배양하여 탈세포화를 시행하였다. 이렇게 탈세포화 실험을 마친 조직은 hematoxylin-eosin (H&E) 염색을 통해 탈세포화의 정도와 세포 외 기질의 보존 정도를 평가하였고, 일부탈세포화된 조직에서는 이종항원면역제거 정도를 파악하는 alpha-Gal 염색과 DAPI 염색을 동시 시행하여 관찰하였다. 결과: Polyethylene glycol이나 peracetic acid를 이용한 방법에서는 탈세포화가 되지 않았다. 단일단계방법으로는 sodium deoxycholate (DOA), sodium dodesyl sulfate (SDS), Triton X-100, SDS와 Triton X-100을 섞은 용액에서, 다단계방법으로는 저장성 완충용액 ${\rightarrow}$ X-100 ${\rightarrow}$ SDS, DOA ${\rightarrow}$ 저장성 완충용액 ${\rightarrow}$ SDS, 저장성 완충용액 ${\rightarrow}$ SDS에서 탈세포화가 이루어 졌다. DOA는 다른 탈세포화 방법에 비해 세포 외 기질의 파괴가 심하였고, 특히 실험온도가 높아질 수록 세포 외 기질의 파괴가 더욱 현저함을 알 수 있었다. 사용되는 화학물질의 종류, 양, 처리시간 및 세포 외 기질의 파괴 정도를 고려하여 지속적으로 재현 가능한 탈세포화에 비교적 적합한 조합 및 조건은 단일단계방법으로 $4^{\circ}C$에서 SDS와 Triton X-100를 섞은 저장성용액에서 24시간 배양하는 방법과, 다단계방법으로 저장성 완충용액과 SDS를 연속적으로 사용하는 방법으로, $4^{\circ}C$에서 $6{\sim}8$시간 이상 저장성 완충용액에 처리한 후, 0.25% SDS가 섞인 저장성 완충용액에 16시간 배양 후 등장성 완충용액에 처리하는 방법이었다. 결론: $4^{\circ}C$에서 SDS 과 Triton X-100을 섞은 저장성 완충용액에서 24시간 배양하는 단일단계방법이나, 저장성완충용과 SDS를 연속적으로 사용하는 다단계 방법을 통해 세포 외 조직을 비교적 잘 보존하면서 적은 수의 탈세포화 용액을 사용하여 효과적인 탈세포화를 얻을 수 있었다.

• Animal cells and systems
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• 제2권2호
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• pp.249-258
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• 1998

Obesity, one of the most common metabolic diseases in industrial countries is characterized by an increase in the number or size of adipocytes. In an effort to create transgenic mouse models for the study of obesity we developed a novel technique in which adipose tissue can be ablated genetically at will, at any specific developmental stage and/or physiological condition, by the treatment of ganciclovir. We made a series of adipocytespecific expression vectors using minimal regulatory regions of brown adipocyte-specific uncoupling protein (UCP-1) gene and adipocyte-specific aP2 gene, and then analyzed their expression characteristics in cultured cell lines. When both constructs pUCP-LacZ and paP2-LacZ were transfected transiently into differentiating 3T3-L1 (pre-while adipocytes) and HIB-1B (pre-brown adipocytes) cell lines in vitro and then monitored by X-gal staining of cells, these regulatory regions were sufficient to show proper differentiation stage-specific expression in adipocvtes. To confirm that adipocytes expressing HSV-TK controlled by these minimal requlatory elements are sufficient to kill themselves with ganciclovir treatment pUCP-TK and paP2-TK expression constructs were transfected stably into HIB-1B and 3T3-L1 cells, respectively, and their ganciclovir sensitivities were tested during in vitro differentiation of cells. As expected more than 80% of cells were dead by the 7th day of treatment with ganciclovir while negative control cells were not affected at all. The data suqqest that the constructed vectors are suitable for obtaining novel obese transqenic models based on a conditional genetic tissue ablation method.

• Journal of Acupuncture Research
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• 제18권2호
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• pp.51-66
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• 2001

The purpose of this morphological studies was to investigate the central neural pathway projecting to the acupoints $B_{62}$ and $K_6$ using the neuroanatomical method following injection of transsynaptic neurotropic virus, pseudorabies virus(PRV-Ba and PRV-Ga) into the $B_{62}$ and $K_6$. After survival times of 96 hours following injection into the twenty rats with PRV-Ba(Bartha strain) and PRV-Ga(Bartha strain, ${\beta}$-galacidodase insertion). They were perfused, and their spinal cord and brain were frozen sectioned($30{\mu}m$). These sections were stained by X-gal histochemical and PRV immunohistochemical staining method, and observed with light microscope. The results were as follows : 1. In spinal cord, overlaped PRV-Ba and PRV-Ga labeled neurons projecting to the $B_{62}$ and $K_6$ were founded in thoracic, lumbar and sacral spinal segments. In thoracic spinal segments, Densely labeled areas were founded in lamina IV, V, VII(intermediolateral nucleus) and X areas. In lumbar segemnts, labeled areas were founded in lamina II, IV, V and X areas. In sacral spinal segments, labeled areas were founded in lamina IV, V and VI areas. 2. In brain, overlaped PRV-Ba and PRV-Ga labeled neurons projecting to the $B_{62}$ and $K_6$ were founded in the $A_1$ noradrenalin cells/$C_1$ adrenalin cells/caudoventrolateral reticular nucleus, rostroventrolateral reticular nuclens, nucleus tractus solitarius, area postrema, raphe obscurus nucleus, raphe paltidus nucleus, raphe magnus nucleus, lateral paragigantoceltular nucleus, lateral rcticular nucleus, gigantocellular nucleus, locus coeruleus, subcoeruleus nucleus, motor trigeminal nucleus, Kolliker-Fuse nucleus, $A_5$ cell group, central gray matter, oculomotor nerve, paraventricular hypothalamic nucleus, median eminence, amygdaloid nucleus, frontal cortex, forelimb area, hindlimb area, 1, 2 areas of parietal cortex and granular and agranular cortex. This results were suggest that overlaped PRV-Ba and PRV-Ga labeled areas projecting to the $B_{62}$ and $K_6$ may be related to the emotional relay pathway in the central autonomic center.

• Journal of the Korean Association of Oral and Maxillofacial Surgeons
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• 제31권4호
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• pp.306-311
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• 2005

Despite advances in surgery, radiotherapy, and chemotherapy, the survival of patients with oral squamous cell carcinoma has not significantly improved over the past several decades. Gene therapy is currently under investigation and shows us new possibility of cancer curing method. This experiment was undergone to find out the cell growth inhibition effect and evidence of apoptosis by HCCS-1(human cervical cancer suppressor-1), one of the candidates of tumor suppressor gene, transducted to human oral cancer cell line. To determine the efficiency of the adenovirus as a gene delivery vector cell line was transducted with LacZ gene and analysed with X-gal staining. Northern blot was performed to confirm the transfection with HSCC-1 gene and cell viability was assessed by cell cytotoxicity assay using cell count kit(CCK). To show the evidence of apoptosis, DNA fragmentation assay and flow cytometry(FACS) were performed. We had successfully construct the recombinant HSCC-1 adenovirus(Ad5CMV-HCCS-1), and importation efficiency was 20% at 2 MOI(multiplicity of infection), 80% at 20 MOI. Northern blot analysis showed that a single 0.6kb mRNA transcript was expressed in Ad5CMV-HCCS-1 transducted cell lines. As a result of CCK, when comparing to control subjects, transducted group showed 50% growth inhibition. In DNA fragmentation assay, according to increasing of MOI, DNA volume was diminished. In FACS analysis, DNA distribution showed fragmentation. This results imply that HCCS-1gene has growth inhibition effect in human oral cancer cell lines through apoptosis induction.

• Maxillofacial Plastic and Reconstructive Surgery
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• 제27권2호
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• pp.103-109
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• 2005

In spite of the ongoing advances, standard therapies for oral cancer still has some limitations in efficacy and in ability to prolong survival rate of advanced disease and result in significant functional defect and severe cosmetic deformity. Currently gene therapy using tumor suppressor gene is considered as a potent candidate for new therapeutic approaches that can improve efficacy and reduce complications. The purpose of this research is to identify the role of adenoviral vector to transfer HCCS-1 tumor suppressor gene in oral cancer cells and to find out whether there is a possibility for it to serve in the field of gene therapy. The human SCC-25 cell line was used for transfection. To determine the efficiency of the adenovirus as a gene delivery vector cell line was transduced with LacZ gene and analysed with X-gal staining. Northern blot was performed to confirm the tranfection with HSCC-1 gene and cell viability was assessed by cell cytotoxicity assay. We had successfully construct the recombinant HSCC-1 adenovirus(Ad5CMV-HCCS-1). DNA extracted from Ad5CMV-HCCS-1 revealed HCCS-1 gene is incorporated. The transduction efficiencies were over than 50% of SCC-25 cells with a MOI of 2 and over 95% with a MOI of 50. Northern blot analysis showed that a single 0.6kb mRNA transcript was expressed in Ad5CMV-HCCS-1 transduced SCC-25 cells. There was no or very low transcription HCCS-1 mRNA in wild and Ad5CMV-LacZ transduced SCC-25 cells. Cells transduced with Ad5CMV-HCCS-1 showed significant growth inhibition. By day 6, Ad5CMV-HCCS-1 treated cell count was decreased to 30% of mock-infected cells, while that of Ad5CMV-LacZ treated cells was 90% of mock-infected cells (p<0.05). Finally, these result suggest that the Ad5CMV-HCCS-1 has potential as a gene therapy tool for oral cancer.

• 한국수정란이식학회지
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• 제17권1호
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• pp.45-53
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• 2002

본 연구는 sperm-mediated gene transfer를 이용하여 ICSI에 의한 형질전환동물 생산의 기초자료로서 활용하기 위해, ICSI에 사용될 정자의 조건과, 그에 따라 적합한 돼지 정자와 외래유전자의 전처리 및 ICSI를 통한 수정을 및 후기 배로의 발달율과 외래유전자의 발현 여부를 조사하여 다음과 같은 결과를 얻었다. ICSI에 이용될 정자의 조건에 따라 정소상체미부정자, 사출정자 및 동결정자를 이용하여 ICSI후 수정율은 각각 72.3%, 64.1% 및 74.1%로 나타나 유의적인 차이를 나타내지 않았으며, 또한 후기배로의 발달율에 있어서도 각각 17.6%, 18.7% 및 15.0%로 나타나 각 처리군간의 유의적인 차이는 나타나지 않았다. 그리고, ICSI후 전기적 자극을 실시한 군과 실시하지 않은 군에서 난자의 활성화에 따른 수정율은 대조구로 이용한 shame injection과 전기적 활성화를 실시하지 않은 군에서 각각 47.1%와 46.3%로 나타나 전기적 활성화를 실시한 군의 79.6%에 비해 유의적인 차이를 나타내었다. 후기배로의 발달율에 있어서도 전기적 활성화를 실시한 군에서는 24.1%로 나타나 전기 적 활성화를 실시하지 않은 군에서의 14.4%와 유의적인 차이를 나타내었다. 그리고 대조구로 이용한 shame injection에 있어서 후기 배로의 발달율은 2.5%로 낮은 결과를 나타내었다. 또한, 정자와 pcDNA LacZ유전자의 처리시 electroporation 방법을 실시하여 ICSI후 난자를 각각 전기적 활성화를 실시한 군과 실시하지 않은 군에 있어서 유전자 발현율은 각각 30.2%와 24.2% 나타났으나, 두 처리군간에 유의적인 차이는 나타나지 않았다. 그러나, 두 군에서 pcDNA LacZ 유전자는 모두 mosaic 발헌 양상을 보였다. 이상의 실험 결과들을 종합해 보면, ICSI에 사용될 수 있는 돼지의 정자는 정소상체미부정자, 사출정자 및 동결정자 모두가 이용 가능하며, ICSI후 추가 전기적 자극에 의한 난자의 활성화가 수정율과 후기 배로의 발달율을 향상시킬 수 있음을 시사하였다. 따라서, 돼지에 있어서 정자의 외래유전자 도입에 대한 정확하고 실용적인 방법은 보고되고 있지는 않은 상태로, 정자와 외래유전자의 처리법을 향상시키기 위하여 다양한 방법으로 많은 연구가 요구된다.