• 약학회지
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• 제31권2호
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• pp.116-125
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• 1987

It is still difficult and time consuming to obtain cDNA sequences that contain the entire nucleotide sequence of the corresponding mRNA. A rapid and high efficient cloning method to obtain full-length cDNA segments is thus developed. The cloning procedure described here consists of the construction of oligo(dT)-tailed vector primer using pWR34 plasmid, polyadenylation of mRNA-cDNA heteroduplex using terminal deoxytransferase, and replacement of MRNA strand with DNA by RNase H and DNA polymerase I. The restriction endonuclease analysis shows that the size of inserted-cDNA is in the range of 1.5~4.0 kb long suggesting that most of cloned cDNA are full-length or nearly full-length cDNA. The plasmid-DNA recombinants obtained were 4$\times$$10^5$~$10^{6}$ per $\mu\textrm{g}$ of rat liver poly (A$^+$)mRNA, which is 4 to 10 fold higher cloning efficiency in comparison to the presently used methods for full-length cDNA cloning. The results indicate that the described cloning system is much simpler, less time consuming, and very efficient cloning method to construct a cDNA library.

• 생명과학회지
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• 제23권6호
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• pp.770-778
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• 2013

본 연구에서는 광양만 해수의 세균군집 다양성의 계절적인 변화를 분석하기 위해 2011년 2월, 5월, 7월, 10월의 4계절에 총 336 균주를 분리하였다. 분리된 미생물의 16S rRNA를 제한효소 Hae III를 이용하여 Amplified Ribosomal DNA Restriction Analysis 를 실시하여 절편 양상을 군집화 시키고, 다양성 지수를 계산하였다. 80%의 유사도 수준에서 40개의 단일 계통형을 포함한 총 101개의 계통형을 얻을 수 있었다. 각 계통형을 대표할 수 있는 139개 균주를 선택하여 16S rRNA 염기서열을 결정한 후 유전자서열을 비교한 결과, 이들 균주는 Proteobacteria, Actinobacteria, Bacteroidetes 및 Firmicutes를 포함한 4개의 문에 속하였다. 모든 계절에 Proteobacteria 문이 최 우점하였고, 겨울과 봄, 가을에는 Bacteroidetes 문, 여름에는 Actinobacteria 문이 차 우점하였다. 과(family) 수준에서는 겨울과 봄에는 Flavobacteriaceae가 우점하였고, 여름과 가을에는 Pseudoalteromonadaceae가 우점하였다. 모든 계절에 Altererythrobacter, Loktanella, Pseudoalteromonas, Vibrio 속(genus)이 관찰되었다. 미생물 군집의 다양성은 가을에 가장 높았으며, 다음으로 봄, 겨울, 여름 순서였다.

• 환경위생공학
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• 제14권4호
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• pp.99-109
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• 1999

Enteropathogenic Yersina enterocolitica is an important cause of human and animal disease. Phenotypic and genotypic characteristics currently used to identify Yersinia enterocolitica are not necessarily sufficient to differentiate pathogenic from non-pathogenic strains or to analyze the epidemiology of yersiniae at a molecular level. To improve the characterization of Yersinia enterocolitica, A total of 65 isolates of Yersinia enterocolitica were examined with bioserotyping, antibiotic susceptibilities, PFGE, PCR-ribotyping. Genomic DNA pattern generated by PFGE are highly specific for different strains of an organism and have significant value in epidemiologic investigations. The PFGE analysis of Not I-digested chromosomal DNA of Y. enterocolitica were performed with a CHEF Mapper(Bio-Rad, USA). Not I generated 19 restriction endonuclease digestion profiles(REDP). PCR-ribotyping, performed with primers complementry to conserved regions of 16S and 23S rRNA gene, generated 13 ribotypes. PCR-ribotyping can be considered a good technich for subtyping strains of Y.enterocolitica.

• 한국식물병리학회지
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• 제11권1호
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• pp.66-72
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• 1995

The coat protein (CP) gene of cucumber mosaic virus-As (CMV-As) strain was engineered for expression in the plant by using the cauliflower mosaic virus 35S transcript regulatory sequences. The CP gene was cloned into an Agrobacterium-derived binary vector. A chimeric gene was constructed by the cDNA of CMV-As CP and plant expression vector pBI121. The clone, pCMAS66, was first introduced into the phagemid vector pSPORT1 for situating sense orientation for translation and making restriction sites in order to re-introduce plant expression vector, pHI121. The resulting subclone pCASCP02 and plant expression vector pBI121 were treated with BamHI-SacI for excising the target gene and removing GUS gene, respectively. After Agrobacterium transformation by freeze-thaw technique, the clone, pCMASCP121-123 which contains sense orientation of the target gene, was selected and confirmed by restriction endonuclease analysis. The CMV-As CP gene was introduced into A. tumefaciens. The results on tobacco plant transformation with the vector system revealed that the system could be successfully introduced and showed high frequency of selection to putative transformations.

• 한국응용곤충학회지
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• 제28권3호
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• pp.105-112
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• 1989

누에(Bombyx mori)와 흰불나방(Hyphantria cunea)으로 부터 분리된 핵다각체병바이러스(nuclear polyhedrosis virus: NPV)를 동정하기 위하여 전자현미경 관찰한 결과, BmNPV 다각체의 크기는 $3 \mu\textrm{m}$ 정도의 18면체로 외형이 균일하였으나, HcNPV는 1.5-$2 \mu\textrm{m}$ 정도이며 부정형이었다. Alkaline protease를 부활화시킨 후 SDS-PAGE한 다각체 단백질의 分子물은 BmNPV가 30 KD, HcNPV는 31 KD인 major band와 이들의 중합체(polymer)로 생각되는 57 KD, 112 KD의 minor band들이 관찰되었다. 또한 virion 단백질을 SDS-PAGE한 후 은염색한 결과, BmNPV는 분자량 9.6~112 KD인 47개의 band, HcNPV 경우는 분자량 9.4~l11 KD인 48개는 band가 관찰되었다. BmNPV와 HcNPV DNA의 제한효소 처이에 의한 전기영동 패턴을 관찰했으며, 각각의 genome 크기는 BmNPV가 약 116.4 Kb, HcNPV의 약 114.6 Kb였다.

• Journal of Microbiology and Biotechnology
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• 제7권4호
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• pp.229-236
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• 1997

A gene, $phbC_{2.4.1}$ encoding poly-3-hydroxybutyric acid (PHB) synthase of Rhodobacter sphaeroides 2.4.1 was cloned by employing heterologous expression in Escherichia coli. R. sphaeroides chromosomal DNA partially digested with MboI was cloned in pUC19 followed by mobilization into E. coli harbouring $phbA,B_{AC}$ in pRK415, which code for ${\beta}$-ketothiolase and acetoacetyl CoA reductase of Alcaligenes eutrophus, respectively. Two E. coli clones carrying R. sphaeroides chromosomal fragment of $phbC_{2.4.1}$ in pUC19 were selected from ca. 10,000 colonies. The PHB-producing colonies had an opaque white appearance due to the intracellular accumulation of PHB. The structure of PHB produced by the recombinant E. coli as well as from R. sphaeroides 2.4.1 was confirmed by [$H^{+}$]-nuclear magnetic resonance (NMR) spectroscopy. Restriction analysis of the two pUC19 clones revealed that one insert DNA fragment is contained as a part of the other cloned fragment. An open reading frame of 601 amino acids of $phbC_{2.4.1}$ with approximate M.W. of 66 kDa was found from nucleotide sequence determination of the 2.8-kb SaiI-PstI restriction endonuclease fragment which had been narrowed down to support PHB synthesis through heterologous expression in the E. coli harbouring $phbA,B_{AC}$. The promoter (s) of the $phbC_{2.4.1}$ were localized within a 340-bp DNA region upstream of the $phbC_{2.4.1}$ start codon according to heterologous expression analysis.

• 한국응용곤충학회지
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• 제34권4호
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• pp.373-377
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• 1995

전국의 토양시료로부터 3가지의 곤충목인, 나비목, 파리목, 딱정벌레목에 속하는 10종의 곤충에 대하여 독성을 보이지 않는 4종의 Bacillus thunngiensis 균주를 분리하였다. 이들 4종의 균주를 각각 NTB-1, NTB-2, NTB-3, NTB-4로 명명하였다. 취상차 현미경과 주사전자현미경을 통해 관찰된 이들 4종 균주의 내독소 단백질 형태는 모두 원형이었으며, 각 균주의 내독소 단백질과 plasmid DNA 특성을 규명하기 위해 단백질 전기영동과 제한효소 분석을 실시하였다. 그 결과 이들 균주의 내독소 단백질과 plasmid DNA pattern은 이미 알려져 있는 무독성 균주들과는 다른 양상을 보여, 기존의 무독성 균주와 다른 새로운 균주임을 알 수 있었다.

• Pediatric Infection and Vaccine
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• 제3권1호
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• pp.76-85
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• 1996

Adenoviruses(Ad) are considered to be second only to rotaviruses as the most significant cause of gastroenteritis in young children in Korea and thus it is essential to know the full spectrum of Ad serotypes routinely present in stool specimens from symptomatic patients. Sixty-six Ad isolates and three questionable ones collected over a 2-year peiord were typed by standard microneutralization, restriction endonuclease digestion and PCR of viral DNA to be able to evaluate these assays comprehensively for their ability to identify Ad associated with gastroenteritis. A total of sixty-one isolates(88.4%) were typed: the predominant types were Ad type 41(Ad41)(26.2%), Ad2(19.7%), Ad40(14.8%), Ad5(9.8%), and Ad7(9.8%) which together accounted for almost 80% of the isolates. The remaining virus isolates were typed as Ad1, 31, 34, 3, 25 and a mixture of 40/41. The incidence of Ad31(4.9%) or Ad3(1.6%) was relatively insignificant. DNA restriction analysis(77.5%) proved to be better than serum neutralization but not so when compared to a PCR-based assay for identification of the enteric Ad serotypes(90%) in stool specimens. In this work, the PCR-based assay was evaluated as a tool for the rapid, yet highly sensitive identification of adenoviral DNA sequences in fresh clinical stool specimens.

• 한국응용곤충학회지
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• 제30권2호
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• pp.144-149
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• 1991

국내에서 분리된 파밤나방 핵다각체병바이러스(Spodoptera exigua nuclear polyhedrosis virus: SeNPV)의 생화학적인 특성을 규명하기 위하여 몇가지 실험을 행하였다. SeNPV는 하나의 envelopeso내에 다수의 nucleocapsid가 존재하는 MNPV(multiple embeded NPV)형태였다. 다각체단백질은 분자량 30kb의 단일 band로 나타났으며, Spodoptera litura NPV와 Bombyx mori NPV의 다각체단백질 항체에 반응하여 뚜렷한 침강선을 형성하였다. 비리온 단백질을 은염색한 결과, 많은 수의 minor band들이 포함된 49개의 band로 나타났으며, 바이러스 DNA를 분리하여 여러종의 제한효소에 의한 대략적인 genome size는 약 110kb 였다.

• 대한수의학회지
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• 제39권1호
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• pp.118-125
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• 1999

Porcine Proliferative Enteropathy(PPE) is an infectious enteric disease and a major cause of economic loss in swine industry due to weight loss, poor growth and sudden death in growing and finishing pigs at 6 to 20 weeks of age. PPE has been diagnosed by clinical signs, syndrom and lesions in the intestine in Korea. However, the diagnostic method had several problems in the detection of infected or carrier pigs. Therefore, in this study, we established the polymerase chain reaction(PCR) which was a fast, specific and sensitive method for identification of Lawsonia intracellularis (L intracellularis). We designed and synthesized primer on the 16S rDNA and p78 gene encoding L intracellularis. Specificity of the method was confirmed by comparison of the PCR results using other enteric bacteria and the study has shown that PCR method was sensitive to detect 1ng of genomic DNA as a template. Identity of the PCR products was confirmed by comparison of pattern of restriction endonuclease analysis with restriction enzyme Hae III and Pst I. Also, the PCR method was applicable to the naturally affected pigs with PPE. Based on the results from this study, the PCR method could be used as a fast and specific diagnostic tool for PPE.