• Genomics & Informatics
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• 제6권2호
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• pp.72-76
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• 2008

Hypoxia-inducible factor $1{\alpha}\;(HIF1{\alpha})$ is a transcription factor that plays a key role in the adaptation of cells to low oxygen stress and oxygen homeostasis. The oxygen-dependent degradation (ODD) domain of $HIF1{\alpha}$ is responsible for the negative regulation of $HIF1{\alpha}$ in normoxia. The interactions of the $HIF1{\alpha}$ ODD domain with partner proteins such as von Hippel-Lindau tumor suppressor (pVHL) and p53 are mediated by two sequence motifs, the N- and C-terminal ODD(NODD and CODD). Multiple sequence alignment with $HIF1{\alpha}$ homologs from human, monkey, pig, rat, mouse, chicken, frog, and zebrafish has demonstrated that the NODD and CODD motifs have noticeably high conservation of the primary sequence across different species and isoforms. In this study, we carried out molecular dynamics simulation of the structure of the $HIF1{\alpha}$ CODD motif in complex with the p53 DNA-binding domain (DBD). The structure reveals specific functional roles of highly conserved residues in the CODD sequence motif of $HIF1{\alpha}$ for the recognition of p53.

• 한국가금학회지
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• 제40권3호
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• pp.223-234
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• 2013

Poultry industry is abounding day by day as it engrosses less cost of investment per bird as compared to large animals. Poultry have the most copious genomic tool box amongst domestic animals for the detection of quantitative trait loci (QTL) and marker assisted selection (MAS). Use of multiple markers and least square techniques for mapping of QTL affecting quality and production traits in poultry is in vogue. Examples of genetic tests that are available to or used in industry programs are documented and classified into causative mutations (direct markers), linked markers in population-wide linkage disequilibrium (LD) with the QTL (LD markers), and linked markers in population wide equilibrium with the QTL (LE markers). Development of genome-wide SNP assays, role of 42 K, 60 K (Illumina) and 600 K (Affymetrix$^{(R)}$ Axim$^{(R)}$) SNP chip with next generation sequencing for identification of single nucleotide polymorphism (SNP) has been documented. Hybridization based, PCR based, DNA chip and sequencing based are the major segments of DNA markers which help in conducting of MAS in poultry. Economic index-marker assisted selection (EI-MAS) provides platform for simultaneous selection for production traits while giving due weightage to their marginal economic values by calculating predicted breeding value, using information on DNA markers which are normally associated with relevant QTL. Understanding of linkage equilibrium, linkage dis-equilibrium, relation between the markers and gene of interest are quite important for success of MAS. This kind of selection is the most useful tool in enhancing disease resistance by identifying candidate genes to improve the immune response. The application of marker assisted selection in selection procedures would help in improvement of economic traits in poultry.

• Journal of Plant Biotechnology
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• 제1권1호
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• pp.46-55
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• 1999

The expressed sequence tags(ESTs) from immature seed of rice, Oryza sativa cv Milyang 23, were partially sequenced and analyzed by homology. As of 1998, the partial sequences of about 6,600 cDNA clones were analyzed from normal and normalized immature seed cDNA libraries. About 2,200 ESTs were putatively identified by BLASTX deduced amino acid sequence homology analysis. About 20% of them were putatively identified as storage proteins. Also the clones were highly homologous to genes involved particularly in starch biosynthesis, glycolysis, signal transduction and defenses. Compared to 35% of redundancy in the ESTs of normal cDNA library, that from the substracted library was 15%. The Korea Rice Genome Network is maintained to provide the updated information of sequences, their homologies and sequence alignments of ESTs. For the stable expression of transgene in rice, diverse vectors were developed for overexpression, targeting and gene dosage effect with transit peptides (Tp) and matrix attachment region (MAR) sequence from chicken lysozyme locus. The rice calli were transformed via Agrobacterium tumefaciens LBA4404(pSB1) with the triparental mating technique and selected by herbicide resistance. The green fluorescent protein(GFP) gene in expression vector under the control of rbcS promoter-Tp was overexpressed upto 10 % of the total soluble protein. In addition, the Tp-sGFP fusion protein was properly processed during translocation into chloroplast. The expression of sGFP in the presence of MAR sequences was analyzed with Northern and immunoblot analysis. All the lines in which sGFP transgene with MAR sequence, showed position independent and copy number-dependent expression, while the lines without MAR showed the varied level of expression with the integration site. Thus the MAR sequence significantly reduced the variation in transgene expression between independent transformants.

• 한국동물위생학회지
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• 제34권1호
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• pp.5-12
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• 2011

Infectious bursal disease (IBD) caused by infectious bursal disease virus (IBDV) is a highly contagious viral disease in chicken. It causes heavy economic loss by immune suppression and high mortality. The IBDV, designated Avibirnavirus in the Family Birnaviridae, has a double-stranded RNA genome formed by two segments, segment A and segment B. Segment A encodes a 108 KDa polypeptide that is self-cleaved to produce pVP2, VP3 and VP4, and later pVP2 is cleaved to VP2. The VP2 contains the antigenic regions responsible for elicitation of neutralizing antibodies and VP3 is a major immunogenic protein of IBDV. In this study, monoclonal antibodies (MAbs) specific for IBDV were produced and characterized. All 15 MAbs were specific for IBDV and did not react with other viruses used in this study. The protein specificity of MAbs was determined by comparing the reactivity patterns of each MAb with IBDV VP2 and VP234 recombinant baculoviruses and Western blot analysis. As a result, 7 MAbs (1F5, 2C8, 2F4, 3C7, 4C3, 6F11, 6G5) and 5 MAbs (2A4, 2G2, 3F5, 3G2, 4F10) were specific for VP2 and VP3, respectively. The protein specificity of 3 MAbs (2B8, 3F7, 3F8) were not determined. Five (2C8, 2F4, 4C3, 6F11, 6G5) of the VP2-specific MAbs had a neutralizing activity against IBDV. Some MAbs reacted with IBDV-infected bursa of Fabricius by indirect fluorescence antibody (IFA) and immunohistochemistry (IHC) assay. The MAbs produced in this study would be used for diagnostic reagents for the detection of IBDV infection.

• Reproductive and Developmental Biology
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• 제30권3호
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• pp.189-194
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• 2006

Sperm-mediated gene transfer(SMGT) can be used to transfer exogenous DNA into the oocyte at fertilization. The main objective of this study was to assess efficiency of transferring mitochondrial DNA(mtDNA) fragment into boar spermatozoa in either presence or absence of liposome and quality of transfected spermatozoa. The mtDNA of chicken liver was isolated and purified by phenol and alkaline lysis extraction, and it was inserted to plasmid. The genome of transfected spermatozoa treated with DNase I was purified by alkaline lysis, and then amplified by the PCR analysis. After electrophoresis, DNA quantitation of each well was calculated by comparison of the band intensity with standard. As a result, exogenous DNA was composed of mtDNA fragment(1.2 kb) and plasmid(2.7 kb). On the other hand, efficiency of transfection by liposome($9.0{\pm}0.34ng/{\mu}l$) in SMGT was higher than that by DNA solution($6.9{\pm}0.53ng/{\mu}l$). However, there was no significant difference. Transfering exogenous DNA into spermatozoa was completed within 90 min of incubation. In another experiment, there were significant (p<0.05) differences between transfected spermatozoa using both DNA solution and DNA/liposome completes with unheated spermatozoa for viability ($70.8{\pm}1.80$ and $68.0{\pm}2.16%$ vs. $83.3{\pm}1.69%$, respectively) and motility($78.7{\pm}1.59$ and $79.3{\pm}2.14%$ vs. $86.7{\pm}1.59%$, respectively). This study indicates that exogenous mtDNA can be efficiently transferred into boar spermatozoa regardless of the presence of liposome, and transfected spermatozoa can also use insemination and in vitro fertilization to generate transgenic pig.

• 생명과학회지
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• 제22권12호
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• pp.1672-1679
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• 2012

본 연구는 육계에서 고밀도 사양체계가 간의 지놈 전사체, 특히 스트레스 및 지방대사 연관 유전자들의 발현에 어떤 영향을 미치는지 알아보기 위하여 실시하였다. 공시된 시험동물의 대조군 사육밀도는 $495cm^2$/수, 고밀도군은 $245cm^2$/수를 35일령까지 유지하였다. 대조구와 비교하여 고밀도 사양 육계에서 체중, 증체량, 사료섭취량이 유의적(p<0.05)으로 감소되는 것으로 나타났다. 폐사율은 고밀도군에서 15.7%로서 대조군(3.7%)에 비해 폐사율이 4.2배 높았다. 육계의 사육밀도에 따른 스트레스관련 유전자 HMGCR, $HSP90{\alpha}$, HSPA5 (GRP78/Bip), DNAJC3, ATF4 등의 발현이 증가하였으며, interferon-${\gamma}$, PDCD4 등의 발현은 감소하였다. Endoplasmic reticulum (ER) stress 관련 HSPA5 (GRP78/Bip), DNAJC3 그리고 ATF4은 유전자들은 고밀도 사양계에서 유전자의 발현이 2-3배 증가함을 보였다. 고밀도 사양은 지방산 합성에 관여하는 효소들(ACSL5, TMEM195, ELOVL6)의 유전자 발현증가와 지방산산화(${\beta}$-oxidatin)에 관여하는 효소들(ACAA1, ACOX1, EHHADH, LOC423347, CPT1A)의 RNA 발현 증가를 유도하였다. 본 연구는 밀사에 의한 스트레스가 닭의 간에서 지방을 합성하기 위한 유전자들의 발현을 증가시키고, 합성된 지방산을 분해하여 에너지를 생산하기 위한 지방산의 산화도 높게 유지하고 있음을 보여주었다. 닭의 주요 지방대사기관인 간에서 외부적 환경인자(사육환경)에 의한 스트레스와 생리적 대사(지방대사 및 소포체 스트레스)가 서로 밀접한 관계가 있음을 분자생물학적 수준에서 확인하였다. 따라서 스트레스저감 사육환경제공 및 친환경 사육방법 도입 등 동물복지를 고려한 가금사양체계가 필요한 것으로 사료된다.

• 한국가금학회지
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• 제50권4호
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• pp.261-266
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• 2023

가축의 골격근은 동물성 단백질 식품으로서 중요한 역할을 하며, 가금육의 소비는 전세계적으로 꾸준히 증가하고 있다. 근육의 형성과 발달에는 근형성조절인자를 포함한 많은 유전자들이 관여하며, 발달 단계에 따라 유전자 발현의 정확한 조절이 필요하다. 본 연구에서는 근육에서 특이적으로 발현하는 유전자를 선발하고, 해당 유전자의 프로모터를 클로닝하고 기능을 분석하였다. 동물의 조직별 유전자 발현을 분석한 결과, 다수의 유전자들이 골격근 특이적인 발현양상을 보였는데, 특히 TNNT3와 TNNC2, MYF6 유전자들은 가금에서도 유사한 양상을 나타냈다. TNNT3, TNNC2, MYF6 유전자의 프로모터 부위를 중합효소연쇄반응을 통해 각각 1.2 kb, 1.03 kb, 1.43 kb씩 증폭하여, 녹색형광단백질 유전자를 포함한 벡터의 앞부분에 삽입하였다. 염기서열 분석 결과, 세 프로모터는 기존에 밝혀진 유전체 서열과 거의 일치함을 확인하였다. QM7 메추리 근육세포주에서 각각의 프로모터를 포함한 벡터를 도입한 결과, 세 프로모터 모두녹색형광단백질을 성공적으로 발현시켰다. 녹색 형광의 밝기는 대조군으로 사용한 CMV-IE 프로모터와 비교 시, 약 7배 정도 어두웠다. 클로닝한 프로모터들에는 230개 이상의 전사인자들이 결합할 수 있을 것으로 예측되었으며, 특히 MYF5나 MYOD, MYOG와 같은 근형성조절인자를 포함한 근육에서 발현하는 다양한 전사인자들이 결합할 수 있을 것으로 예측되었다. 이 프로모터들은 가금의 근육세포에서 유전자 발현을 유도하는 연구에 활용이 가능할 것이며, 추후연구를 통해 프로모터 부위별 발현 조절 기능 연구가 필요할 것으로 사료된다.

• 한국식품위생안전성학회지
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• 제27권2호
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• pp.146-151
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• 2012

본 연구에서는 분자생물학적 방법을 통한 식육추출가공품의 사용원료 확인을 위해 효율적인 유전자 추출 방법을 검토하였다. 가공식품의 원료성분 확인을 위하여 종 특이 프라이머를 이용하였으며, 대상 식품원료로는 소, 돼지, 닭을 주원료로 가공된 식육추출가공품 13종을 선정하였다. 선정된 시료는 제품유형에 따라 액상, 소스, 분말류로 구분하고 원심분리 등의 전처리를 추가하거나 추출유전자의 증폭을 위하여 Whole Genome Amplification (WGA)를 실시한 뒤 유전자증폭 후 전기영동하여 예상되는 PCR 산물의 생성유무를 확인하였다. PCR을 실시한 결과 액상형태 식육 추출가공품의 경우에는 1 ml을 취하여 원심분리 과정을 통해 유전자를 추출 하였을 때 사용원료 확인이 가능하였으며, 소스형태 식육추출가공품의 경우 유전자 추출 후 WGA 과정을 추가로 시행하여야 사용원료확인이 가능하였다. 분말형태 식육추출가공품의 경우에는 추가의 전처리 과정이나 WGA 과정이 필요하지 않았다. 본 연구에서 검토된 유형별 유전자추출법은 식육추출가공품의 유전자추출을 통한 사용원료확인이 가능함을 확인하였으며, 향후 식육추출 가공품 중 사용원료의 진위여부 판별에 활용이 가능할 것으로 판단된다.