• BMB Reports
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• 제40권5호
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• pp.625-635
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• 2007

The enzyme squalene synthase (EC 2.5.1.21) catalyzes a reductive dimerization of two farnesyl diphosphate (FPP) molecules into squalene, a key precursor for the sterol and triterpene biosynthesis. A full-length cDNA encoding squalene synthase (designated as TcSqS) was isolated from Taxus cuspidata, a kind of important medicinal plants producing potent anti-cancer drug, taxol. The full-length cDNA of TcSqS was 1765 bp and contained a 1230 bp open reading frame (ORF) encoding a polypeptide of 409 amino acids. Bioinformatic analysis revealed that the deduced TcSqS protein had high similarity with other plant squalene synthases and a predicted crystal structure similar to other class I isoprenoid biosynthetic enzymes. Southern blot analysis revealed that there was one copy of TcSqS gene in the genome of T. cuspidata. Semi-quantitative RT-PCR analysis and northern blotting analysis showed that TcSqS expressed constitutively in all tested tissues, with the highest expression in roots. The promoter region of TcSqS was also isolated by genomic walking and analysis showed that several cis-acting elements were present in the promoter region. The results of treatment experiments by different signaling components including methyl-jasmonate, salicylic acid and gibberellin revealed that the TcSqS expression level of treated cells had a prominent diversity to that of control, which was consistent with the prediction results of TcSqS promoter region in the PlantCARE database.

• BMB Reports
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• 제39권3호
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• pp.297-303
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• 2006

As lipolytic enzymes, GDSL lipases play an important role in plant growth and development. In order to identify their functions and roles, the full-length cDNA of a GDSL lipase gene, designated BnLIP2, was isolated from Brassica napus L. BnLIP2 was 1,300 bp long, with 1,122 bp open reading frame (ORF) encoding 373 amino acid residues. Sequence analysis indicated that BnLIP2 belonged to GDSL family. Southern blot analysis indicated that BnLIP2 belonged to a small gene family in rapeseed genome. RT-PCR analysis revealed that BnLIP2 was a tissue-specific expressing gene during reproductive growth and strongly expressed during seed germination. BnLIP2 expression could not be detected until three days after germination, and it subsequently became stronger. The transcript of this gene was deficient in root of seedlings growing at different stages. When juvenile seedlings were treated by methyl jasmonate (MeJ), salicylic acid (SA) and naphthalene acetic acid (NAA), BnLIP2 expression could not be induced in root. Our study implicates that BnLIP2 probably plays an important role in rapeseed germination, morphogenesis, flowering, but independent of root growth and development.

• 한국양식학회지
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• 제17권1호
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• pp.1-7
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• 2004

A rainbow trout uncoupling protein 3 (UCP3) cDNA clone, encoding a 310 amino acid protein, was cloned and sequenced from a liver cDNA library. Two different splice variants designated UCP3-vl and UCP3-v2, were identified through liver cDNA library screening using rainbow trout UCP3 cDNA clone as a probe. UCP3-vl has 3 insertions in the UCP3 cDNA: the first insertion (133 bp), the second (141 bp), and the third (370 bp) were located 126 bp, 334 bp and 532 bp downstream from the start codon, respectively. UCP3-v2 contained a single insertion, identical in sequence and location to the second insertion of UCP3-vl. UCP3, a mitochondrial protein, functions to modulate the efficiency of oxidative phosphorylation. UCP3 has been detected from heart, testis, spinal cord, eye, retina, colon, muscle, brown adipose tissue and white adipose tissue in mammalian animals. Human and rodent UCP3s are highly expressed in skeletal muscle and brown adipose tissue, while they show weak expression of UCP3 in heart and white adipose tissue. In contrast to mammalian studies, RT-PCR and Southern blot analysis of the rainbow trout demonstrated that UCP3 is strongly expressed in liver and heart. UCP3, UCP3-vl, and UCP3-v2 all contain an Ava III short interspersed element (SINE), located in the 3'untraslated region (UTR). PCR using primers from the Ava III SINE and the UCP3 3'UTR region indicates that the UCP3 cDNA is structurally conserved among salmonids and that these primers may be useful for salmonid species genotyping.

• 원예과학기술지
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• 제29권6호
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• pp.623-632
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• 2011

본 연구는 배추에서 항암물질 PEITC의 함량을 높이기 위하여 PEITC 대사과정에서 관련 유전자인 myrosinase (MYR)와 Glutathione S-transferase(GST) 유전자를 분리하고 Agrobacterium tumefacien 형질전환 방법을 통하여 유전자 발현을 조절하였다. 분리된 MYR과 GST의 cDNA는 각각 1647bp와 624bp임을 확인하였고 pET system으로 단백질의 발현을 확인하였다. 형질전환을 위해서 MYR-과발현 벡터와 GST-발현억제 벡터를 제작하였으며 이를 이용하여 배추에 형질전환한 후 PCR 검정을 통해 MYR-과발현 벡터로 형질전환된 개체(IMS) 13개체를 GST-발현억제 벡터로 형질전환된 개체(IGA) 5개체를 선발하였다. 선발된 $T_0$ 개체는 $T_1$ 세대로 진전시켰으며 $T_1$ 형질전환 계통의 서던분석 결과 배추 genome내로 1-4 copy의 T-DNA가 삽입된 것을 확인하였다. 유전자 발현양을 real-time RT PCR로 조사한 결과 IMS는 발현량이 1.03-4.25배 증가하였고 IGA는 26.42-42.22배 감소하였다. IMS와 IGA의 각 계통에서 PEITC의 농도를 GC-MS 방법을 이용하여 확인한 결과 IMS는 PEITC 함량이 형질전환이 되지 않은 대조군에 비해 최대 4.86배까지 증가한 계통을 확인하였고 IGA는 최대 3.89배까지 증가된 계통을 확인하였다. 최종적으로 본 연구를 통하여 항암물질 PEITC량의 증가를 보인 형질전환계통 IMS 1, 3, 5, 12, 15 및 IGA 1, 2, 4를 선발하였다.

• 원예과학기술지
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• 제30권2호
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• pp.162-170
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• 2012

스프레이 국화품종 'Argus'와 감마선 조사에 의해 화색변이가 일어난 돌연변이체의 꽃잎으로부터 안토시아닌 생합성 경로에서 중요한 역할을 담당하는 신규 $DgF3'H$의 전장 cDNA와 genomic DNA를 분리하였다. 전장 cDNA는 1,527bp(509 아미노산)의 ORF를 포함하고 있으며, 원품종 'Argus'와 화색변이체 사이의 염기서열 상동성은 97% 이상을 나타내었다. Genomic DNA의 크기는 야생형 'Argus'에서 3,831bp이었고, 3가지 화색 변이체에서는 3,828부터 3,838bp의 크기를 나타내었다. $DgF3'H$ 유전자는 세 개의 exon사이에 두개의 intron을 갖고 있는 구조이고, 3'과 5' UTR 부분을 제외한 intron의 크기는 야생형 'Argus'에서 2,157bp이지만 3가지 화색 변이체에서는 2,155부터 2,159bp의 크기를 갖고 있었다. 이것은 감마선 조사에 의해 intron 부분의 유전자가 결실 또는 삽입된 것으로 추정된다. Southern 분석 결과 국화의 genome 내에서는 복수의 F3'H 유전자를 갖는 것이 확인되었다. $DgF3'H$ 유전자의 발현 정도를 분석한 결과, 연분홍의 'Argus'와 두 개의 보라색 변이체(AM1 and AM3)에서 높게 발현되었으나 흰색 변이체(AM2)에서는 매우 약하게 발현되었으며, 염기서열 변이에 의한 F3'H 유전자의 구조적 차이가 화색의 변이에 관련된 것으로 추정되었다. 국화 'Argus' 및 화색 변이체를 이용하여 본 연구에서 분리한 신규 F3'H 유전자의 구조 및 유전자 발현 등을 포함하는 유전정보들은 화색 변이의 유전적 기작을 밝히는데 중요한 자료로 이용될 것으로 기대되나 향후 다른 유전적 발현요소들이 국화의 F3'H 유전자의 발현에 관여하는지에 관한 추가적인 연구가 필요하다고 하겠다.

• 한국잡초학회지
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• 제18권3호
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• pp.205-213
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• 1998

세계적으로 중요한 식량자원인 감자에 제초제 저항성 형질을 도입한다면, 노지재배가 가능하여 노동력과 인건비를 줄일 수 있을 뿐만 아니라 비닐멀칭 방법의 부산물인 폐비닐에 의한 환경오염을 줄일 수 있는 매우 효과적인 방법이다. 그러나 형질전환식물체의 선발시 일반적으로 사용해온 항생제 내성 표지유전자는 효과적으로 형질전환체를 선발할 수 있는 장점을 가지나 항생제 내성 표지유전자들이 환경중에 노출되었을 때의 안전성 문제, 그리고 일반 소비자들이 항생제 표지유전자를 이용한 형질전환체에 대해 거부감이 느껴지게 할 수 있다는 문제점이 존재한다. 이러한 문제점들은 항생제 내성 표지유전자를 제거하거나 새로운 표지유전자로 대체하는 방법을 사용하여 해결할 수 있을 것으로 생각된다. 따라서 본 실험의 목적은 비선택성 제초제 bialaphos에 저항성을 가지는 phosphinothricin acetyltransferase(PAT) gene을 감자에 도입하는데 있어 항생제 표지 유전자를 사용하지 않는 선발체계를 개발하고자 하였다. 감자 식물체의 재분화는 IBA 0.1mg/L + BA 0.5mg/L를 첨가한 MS배지에서 하였다. 또한 형질전환을 위해 단독 PAT 유전자만을 가지는 pDY502 vector를 재조합하였으며, 재조합된 vector들은 disarmed 된 Agrobacterium MP90에 도입하여 감자의 형질전환에 이용하였다. 형질전환은 강자의 잎과 줄기절편체를 상기 실험에서 재 조합된 vector를 함유한 A. tumefaciens MP90과 공동배양하는 방법으로 수행하였다. PAT 유전자를 표지유전자로 이용하여 bialaphos에 저항성을 가진 감자를 개발하고자 다양한 농도의 bialaphos를 함유한 재분화배지에 감자절편체를 치상하여 내성을 조사한 결과 대조구의 감자절편체가 모두 고사하는 bialaphos 5mg/L를 선발조건으로 하였다. 이와 같은 선발 조건에서 Agrobacterium과 공동 배양한 절편체를 선발배지에 치상한 후 3-4주 정도가 경과하면 shoot가 유기되었으며, 선발배지에서 유기된 shoot의 정단부위를 lcm정도로 잘라 bialaphos가 20mg/L 첨가된 선발배지로 옮겨 2차 선발을 하였다. 형질전환체의 확인은 2차 선발배지에서 선발된 식물체를 대상으로 하였으며, 먼저 PCR반응을 이용하여 도입 유전자의 증폭을 확인하였고, Southern blot을 실시하여 유전자의 도입을 확인하였다. 따라서 PAT 유전자를 감자 형질전환의 표지유전자로 활용할 수 있었으며, 아울러 항생제 표지유전자가 없는 제초제 저항성 형질전환 감자를 획득할 수 있었다.

• Reproductive and Developmental Biology
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• 제38권2호
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• pp.71-77
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• 2014

The specific genetic modification in porcine somatic cells by gene targeting has been very difficult because of low efficiency of homologous recombination. To improve gene targeting, we designed three kinds of knock-out vectors with ${\alpha}1,3$-galactosyltransferase gene (${\alpha}1,3$-GT gene), DT-A/pGT5'/neo/pGT3', DT-A/NLS/pGT5'/neo/pGT3' and pGT5'/neo/ pGT3'/NLS. The knock-out vectors consisted of a 4.8-kb fragment as the 5' recombination arm (pGT5') and a 1.9-kb fragment as the 3' recombination arm (pGT3'). We used the neomycin resistance gene (neo) as a positive selectable marker and the diphtheria toxin A (DT-A) gene as a negative selectable marker. These vectors have a neo gene insertion in exon 9 for inactivation of ${\alpha}1,3$-GT locus. DT-A/pGT5'/neo/pGT3' vector contain only positive-negative selection marker with conventional targeting vector. DT-A/NLS/pGT5'/neo/pGT3' vector contain positive-negative selection marker and NLS sequences in upstream of 5' recombination arm which enhances nuclear transport of foreign DNA into bovine somatic cells. pGT5'/neo/pGT3'/NLS vector contain only positive selection marker and NLS sequence in downstream of 3' recombination arm, not contain negative selectable marker. For transfection, linearzed vectors were introduced into porcine ear fibroblasts by electroporation. After 48 hours, the transfected cells were selected with $300{\mu}g/ml$ G418 during 12 day. The G418-resistant colonies were picked, of which 5 colonies were positive for ${\alpha}1,3$-GT gene disruption in 3' PCR and southern blot screening. Three knock-out somatic cells were obtained from DT-A/NLS/ pGT5'/neo/pGT3' knock-out vector. Thus, these data indicate that gene targeting vector using nuclear localization signal and negative selection marker improve targeting efficiency in porcine somatic cells.

• Molecules and Cells
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• 제26권6호
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• pp.536-547
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• 2008

Anthocyanidin synthase (ANS, leucoanthocyanidin oxygenase), a 2-oxoglutarate iron-dependent oxygenase, catalyzed the penultimate step in the biosynthesis of the anthocyanin class of flavonoids, from the colorless leucoanthocyanidins to the colored anthocyanidins. The full-length cDNA and genomic DNA sequences of ANS gene (designated as GbANS) were isolated from Ginkgo biloba for the first time. The full-length cDNA of GbANS contained a 1062-bp open reading frame (ORF) encoding a 354-amino-acid protein. The genomic DNA analysis showed that GbANS gene had three exons and two introns. The deduced GbANS protein showed high identities to other plant ANSs. The conserved amino acids (H-X-D) ligating ferrous iron and residues (R-X-S) participating in 2-oxoglutarate binding were found in GbANS at the similar positions like other ANSs. Southern blot analysis indicated that GbANS belonged to a multi-gene family. The expression analysis by real-time PCR showed that GbANS expressed in a tissue-specific manner in G. biloba. GbANS was also found to be up-regulated by all of the six tested abiotic stresses, UV-B, abscisic acid, sucrose, salicylic acid, cold and ethylene, consistent with the promoter region analysis of GbANS. The recombinant protein was successfully expressed in E. coli strain with pET-28a vector. The in vitro enzyme activity assay by HPLC indicated that recombinant GbANS protein could catalyze the formation the cyanidin from leucocyanidin and conversion of dihydroquercetin to quercetin, suggesting GbANS is a bifunctional enzyme within the anthocyanidin and flavonol biosynthetic pathway.

• Asian Pacific Journal of Cancer Prevention
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• 제16권15호
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• pp.6769-6772
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• 2015

Background: High risk human papillomaviruses (HPVs) are the leading cause of cervical cancer (CC) and Pap smear screening has not been successful in preventing CC in Tunisia. HPV vaccination that targets HPV16 and 18 offers a new efficient prevention tool. Identification of HPV types in CC is thus essential to determine the impact of HPV vaccine implementation. The aim of this study is to provide specific data from Tunisia. Materials and Methods: A total of 89 histological confirmed paraffin embedded samples isolated from patients with CC diagnosed between 2001 and 2011 were collected from five medical centres from Northern and Southern Tunisia. HPV DNA was detected using a nested PCR (MY09/MY11-GP5+/GP6+) and genotyping was assessed using a reverse blot line hybridisation assay that enables the detection of 32 HPV types. Results: HPV DNA was detected in all samples. Twelve high risk types were detected; HPV16 and/or 18 were predominant, accounting together for 92.1% of all the CC cases (HPV16: 83.1%). Single infections accounted for 48.8% of the cases and were mostly linked to HPV 16 (32.6%) and less frequently to HPV 18 (2.4%). The other high risk HPV single infections were linked to HPV 35 (4.6%), 45 (4.6%), 58 (2.3%) and 59 (2.3%). Multiple infections with mixing of 2 to 4 genotypes predominately featrued HPV16 and/or 18 with HPV 35 and 45 (96.6 %) and less frequently with HPV 59, 40, 66, 73 and 58. There was no statistically significant variation in the relative distribution of HPV types with age. Conclusions: These results strongly indicate that prophylactic HPV vaccines can have a major impact in preventing CC in Tunisia.

• BMB Reports
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• 제41권2호
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• pp.112-118
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• 2008

Camptothecin is an anti-cancer monoterpene indole alkaloid. The gene encoding 1-hydroxy-2-methyl-2-(E)-butenyl 4-diphosphate reductase (designated as CaHDR), the last catalytic enzyme of the MEP pathway for terpenoid biosynthesis, was isolated from camptothecin-producing Camptotheca acuminata. The full-length cDNA of CaHDR was 1686 bp encoding 459 amino acids. Comparison of the cDNA and genomic DNA of CaHDR revealed that there was no intron in genomic CaHDR. Southern blot analysis indicated that CaHDR belonged to a low-copy gene family. RT-PCR analysis revealed that CaHDR expressed constitutively in all tested plant organs with the highest expression level in flowers, and the expression of CaHDR could be induced by 100 ${\mu}M$ methyl-jasmonate (MeJA), but not by 100 mg/L salicylic acid (SA) in the callus of C. acuminata. The complementation of CaHDR in Escherichia coli ispH mutant MG1655 demonstrated its function.