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Kim, Dongbin,Kim, TaeWan,Jin, Yinhua,Mun, Jihun,Lim, In-Tae,Kim, Ju-Hwang,Kim, Taesung,Kang, Sang-Woo The Korean Vacuum Society 2016 Applied Science and Convergence Technology Vol.25 No.2
The surface flatness of metal meshes in a deflector of particle beam mass spectrometer (PBMS) required ideally flat, and this can specify the particle trajectories which goes through the detector. In this research, charged particle current was measured using the different surface roughness deflectors. NaCl particles were generated monodispersed in its size by using differential mobility analyzer and the whole processes were followed the way calibrating PBMS. The results indicate that the mesh surface morphology in the deflector can affect to the particle size and the concentration errors, and sensitivity of PBMS.
효율적인 Metagenomic Library의 제작 방법 탐구
임동빈,Lim Dongbin 한국미생물학회 2004 미생물학회지 Vol.40 No.4
I investigated an effective way to generate a metagenomic library from DNA prepared from environental samples. The sizes of DNA extracted from environmental samples were usually in the range of 10 to 100 kbp as estimated from $0.4\%$ agarose gel electrophoresis. Because of this small size, a fosmid, rather than BAC, was chosen as a vector. It was found that, for the successful generation of metagenomic library, the selection of DNA with the sized of about 40 kbp was critical and, therefore, a simple agarose gel electrophoresis system was developed to select this size of DNA. By the procedure described in this report, I obtained metagenomic libraries containing 25,000 fosmid clones, which corresponded to 1,000 Mb of metagenomic DNA. 자연계에 존재하는 미생물의 대부분이 배양이 불가능하다는 것이 밝혀진 이후, 자연계의 시료로부터 직접 유전자를 클로닝하여 유용유전자를 발굴하는 메타제놈(metagenome) 이용 방법이 주목을 받게 되었다. 그러나 실제로 오염이 심한 환경시료로부터 DNA를 추출하여 유용한 메타제놈 라이브러리(metagenomic library)를 제작하기란 쉽지 않은 일이다. 따라서 본 연구에서는 실제 메타제놈 라이브러리를 제작할 때 만나는 기술적 문제점에 대한 해결 방법을 탐구하였다. 메타제놈 라이브러리 제작에는 fosmid vector가 가장 편리하였으며, 성공적인 라이브러리제작에는 fosmid vector에 클로닝이 가능한 40 kbp 크기의 DNA 조각을 얻는 과정이 중요함을 알았다. 여러 실험 조건을 종합적으로 검사한 후 메타제놈 라이브러리 제작에 대한 최적 방법을 제사하였다.
Comparisons of Recombinant Protein Expression in Diverse Natural Isolates of Escherichia coli
Jung, Yuna,Lim, Dongbin Korean Society for Molecular Biology 2008 Molecules and cells Vol.25 No.3
We assessed heterologous protein expression in 64 strains obtained from the Escherichia coli Reference (ECOR) collection, a collection representing diverse natural E. coli populations. A plasmid generating a glutathione S-transferase and plant carbonic anhydrase fusion protein (GST-CA) under the control of the tac promoter was introduced into the ECOR strains, and the quantity of the fusion protein was determined by SDS-PAGE. The foreign protein was generated at various levels, from very high (40 strains, high producers) to very low (six strains, low producers). Immunoblotting showed that the high producers expressed approximately 250 - 500 times more GST-CA protein than the low producers. The results of semi-quantitative RT-PCR showed that the low producers generated mRNA levels comparable to those of the high producers, thereby suggesting that, at least in this case, inefficient translation is a major cause of the low production. We introduced a different plasmid, which expressed a maltose binding protein and plant guanylate kinase fusion protein (MBP-GK) into the six low producers. Interestingly, five of these expressed MBP-GK at very high levels. Thus, we conclude that the production of a particular protein from an expression vector can vary considerably, depending on the host strain. Strains in the ECOR collection could function as useful alternative hosts when a desired level of protein expression is not obtained from commonly used strains, such as E. coli K12 or B derivatives.
Compiling Multicopy Single-Stranded DNA Sequences from Bacterial Genome Sequences
Yoo, Wonseok,Lim, Dongbin,Kim, Sangsoo Korea Genome Organization 2016 Genomics & informatics Vol.14 No.1
A retron is a bacterial retroelement that encodes an RNA gene and a reverse transcriptase (RT). The former, once transcribed, works as a template primer for reverse transcription by the latter. The resulting DNA is covalently linked to the upstream part of the RNA; this chimera is called multicopy single-stranded DNA (msDNA), which is extrachromosomal DNA found in many bacterial species. Based on the conserved features in the eight known msDNA sequences, we developed a detection method and applied it to scan National Center for Biotechnology Information (NCBI) RefSeq bacterial genome sequences. Among 16,844 bacterial sequences possessing a retron-type RT domain, we identified 48 unique types of msDNA. Currently, the biological role of msDNA is not well understood. Our work will be a useful tool in studying the distribution, evolution, and physiological role of msDNA.
Shin, Sun Woo,Lim, Yu jin,Bae, Hyeona,Kim, Jihu,Cho, ARom,Park, Jinho,Lee, Dongbin,Jung, Dong-In,Kim, Sang-ki,Yu, DoHyeon The Korean Society of Veterinary Science 2021 大韓獸醫學會誌 Vol.61 No.3
Canine T-zone lymphoma (TZL) is a mature T-cell lymphoma in dogs. The diagnosis and sub-classification are impossible without biopsy or immunophenotyping by flow cytometry. An 11-year-old, spayed, female Golden Retriever presented with lymph node enlargement. Clinical examination was consistent with canine multicentric lymphoma. However, immunophenotyping revealed positive for CD3, CD4, CD5, CD8, CD21, TCRαβ, and MHCII but negative for CD34, CD45, CD79a, and TCRγδ. Histopathology revealed lymphocytes expanding to the cortex-preserving architecture and thinning of the nodal capsule, and CD3 positive but PAX-5 negative. Owing to the indolent nature of TZL, careful monitoring approach without clinical intervention was utilized.
정혜임,임동빈,Jung, Hyeim,Lim, Dongbin 한국미생물학회 2016 미생물학회지 Vol.52 No.4
대장균에서 6개의 Leu 코돈중 가장 흔한 코돈은 CUG이다. 이 코돈을 인식하는 tRNA는 4개의 유전자에 의해 합성되는데, leuPQV와 leuT 2개의 locus로 나누어져 있다. 이 CUG를 인식하는 모든 tRNA가 결핍된 균주를 만들기 위해, 우선 leuPQV가 삭제된 균주(${\Delta}leuPQV$)와, leuT의 anticodon CAG를 GAG로 돌연변이시킨 균주[$Km^R$, $leuT^*$(GAG)]를 각각 만들었다. 이 두 돌연변이 유전자를 모으기 위해 ${\Delta}leuPQV$ 균주를 recipient로, $leuT^*$(GAG) 균주를 donor로하는 transduction을 수행한 결과, 콜로니 크기가 큰 것과 작은 것 두 종류의 transductant를 얻었다. PCR 후 염기서열 분석 결과 큰 콜로니는 예측한 recombinant로 판명됐으나, 작은 콜로니는 donor와 recipient 염색체 간의 상호교환재조합(reciprocal recombination)으로는 설명이 되지 않는, 돌연변이 유전자[$leuT^*$(GAG)]와 야생형 유전자(leuT(CAG)]를 모두 가진 균주로 밝혀졌다. 이 heterozygous diploid는 광학현미경으로 관찰시 세포의 형태와 크기에서 특이점이 발견되지 않았으나, 영양배지에서 야생형에 비해 생장이 한참 느리면서, 선형생장곡선(linear growth curve)이라는 예측하지 못한 생장특성을 보였다. 이 2배체 균주는 선택배지에서는 항상 작은 균일한 콜로니를 형성하였으나, 배지에 선택항생제 없을 경우, $leuT^*$(GAG) 유전자형 세포와 leuT(CAG) 유전자형 세포로 분리가 일어났다. 우리의 결과를 종합해볼 때, 이 2배체 균주는, $leuT^*$(GAG)와 leuT(CAG) 부분만 2배체로 갖는 부분이배체(merodiploid)라기 보다는, $leuT^*$(GAG)와 leuT(CAG)가 서로 다른 염색체에 있는 완전이배체라는 모델을 지지했다. 우리는 이러한 2배체가 어떻게 생성되었으며, 어떻게 분리되는지, 또 이 균주는 왜 선형생장곡선을 보이는지 등에 대한 모델을 토론하였다. Among 6 leu codons, CUG is the most frequently used codon in E. coli. It is recognized by leu-tRNA(CAG) encoded by four genes scattered on two chromosomal loci (leuT and leuPQV ). In the process of constructing a strain with no functional leu-tRNA (CAG) gene on chromosome, we made two mutant strains separately, one on leuPQV locus (${\Delta}leuPQV$), and the other on leuT locus [$leuT^*$(GAG)], where the anticodon of leuT was changed from CAG to GAG, thereby altering its recognition codon from CUG to CUC. We attempted to combine these two mutations by transduction using $leuT^*$(GAG) strain as a donor and ${\Delta}leuPQV$ strain as a recipient. Large and small colonies appeared from this transduction. From PCR and DNA sequencing, large colony was confirmed to be the reciprocal recombinant as expected, but the small colonies contained both mutant $leuT^*$(GAG) and wild type leuT (CAG) genes in the cell. This heterozygous diploid strain did not show any unusual morphology under microscopic observation, but, interestingly, it showed a linear growth curve in rich medium with much slower growth rate than wild type cell. It always formed homogenous small colonies in the selection medium, but, when there was no selection, it readily segregated into $leuT^*$(GAG) and leuT (CAG). From these observations, we suggested that the strain with both $leuT^*$(GAG) and leuT (CAG) genes was not a partial diploid (merodiploid), but a full diploid cell having two different chromosomes. We proposed a model explaining how such a heterozygous diploid cell was formed and how and why its growth showed a linear growth curve.