• 제목/요약/키워드: C Library

검색결과 1,222건 처리시간 0.028초

국립대학교 도서관 발전방향에 관한 연구 - C대학 도서관을 중심으로 - (A Study on the Development Direction of National University Library - A Case Study of C National University Library -)

  • 서진원
    • 한국문헌정보학회지
    • /
    • 제35권2호
    • /
    • pp.133-149
    • /
    • 2001
  • 본 논문은 국립대학인 C대학도서관의 사례연구이다. C대학의 특성과 대학도서관의 변화를 살펴보고 이에 따른 C대학도서관의 발전방향을 제시하였다. C대학도서관의 활동을 이용자에 대한 봉사를 기준으로 직접봉사활동과 간접봉사 활동으로 구분하였으며 그 아래에서 세분하여 대학도서관의 활동이 대학의 발전에 어떻게 기여할 수 있을 것인가를 논하였다.

  • PDF

방사무늬 김의 cDNA Library 제조 및 분석 (Construction and Analysis of cDNA Library from Porphyra yezoensis)

  • 서수분;이은경;김영진
    • 생명과학회지
    • /
    • 제9권5호
    • /
    • pp.531-536
    • /
    • 1999
  • As an attempt to preserve resources in marine biological organisms, we first constructed a cDNA library from the red alga Porphyra yezoensis. The library construction method from P. yezoensis consists of three steps; those include protoplast presparation, RNA isolation, and phage library construction. Protoplast was prepared in order to remove much of the carbohydrate compounds which are characteristics of algal cell walls. Carbohydrate contamination in the purified RNA may inhibit further enzyme reactions, those carbohydrates should be removed. RNA samples prepared from protoplast still seemed to contain residual amount of carbohydrate because mRNA isolation with conventional method failed. We therefore developed a method with Poly ATtract mRNA isolation system. The constructed phage library was tested by analyzing cDNA insert in phage vector from randomly picked ten independent white plagues. All of the phages contained cDNA inserts with sizes ranging 0.5kb and 2.0kb.

  • PDF

실시간 운영체계 Q+를 위한 C 표준 라이브러리 설계 및 구현 (The Design and Implementation of C Standard Library for RTOS Q+)

  • 김도형;박승민
    • 정보처리학회논문지A
    • /
    • 제8A권1호
    • /
    • pp.1-8
    • /
    • 2001
  • This paper describes the design and implementation of C standard library for real-time operating system Q+, that is being developed for the internet appliance. The C library in the real-time operating system should be defined according to the standard interface and support the concurrent execution of threads. The implemented C standard library is reentrant and follows POSIX.l standard interface. And, the C standard library functions, which are adequate to the Q+ application and commonly provided by commercial real-time operating systems, are selected among POSIX.l standard functions. The C standard library is implemented on the Q+ kernel and D-TV set-top box according to the implementation sequence, which is determined by analyzing the relation of function calls.

  • PDF

Construction of a High-Quality Yeast Two-Hybrid Library and Its Application in Identification of Interacting Proteins with Brn1 in Curvularia lunata

  • Gao, Jin-Xin;Jing, Jing;Yu, Chuan-Jin;Chen, Jie
    • The Plant Pathology Journal
    • /
    • 제31권2호
    • /
    • pp.108-114
    • /
    • 2015
  • Curvularia lunata is an important maize foliar fungal pathogen that distributes widely in maize growing area in China, and several key pathogenic factors have been isolated. An yeast two-hybrid (Y2H) library is a very useful platform to further unravel novel pathogenic factors in C. lunata. To construct a high-quality full length-expression cDNA library from the C. lunata for application to pathogenesis-related protein-protein interaction screening, total RNA was extracted. The SMART (Switching Mechanism At 5' end of the RNA Transcript) technique was used for cDNA synthesis. Double-stranded cDNA was ligated into the pGADT7-Rec vector with Herring Testes Carrier DNA using homologous recombination method. The ligation mixture was transformed into competent yeast AH109 cells to construct the primary cDNA library. Eventually, a high qualitative library was successfully established according to an evaluation on quality. The transformation efficiency was about $6.39{\times}10^5$ transformants/$3{\mu}g$ pGADT7-Rec. The titer of the primary cDNA library was $2.5{\times}10^8cfu/mL$. The numbers for the cDNA library was $2.46{\times}10^5$. Randomly picked clones show that the recombination rate was 88.24%. Gel electrophoresis results indicated that the fragments ranged from 0.4 kb to 3.0 kb. Melanin synthesis protein Brn1 (1,3,8-hydroxynaphthalene reductase) was used as a "bait" to test the sufficiency of the Y2H library. As a result, a cDNA clone encoding VelB protein that was known to be involved in the regulation of diverse cellular processes, including control of secondary metabolism containing melanin and toxin production in many filamentous fungi was identified. Further study on the exact role of the VelB gene is underway.

Construction of a cDNA library of Aphis gossypii Glover for use in RNAi

  • KWON, HyeRi;KIM, JungGyu;LIM, HyounSub;YU, YongMan;YOUN, YoungNam
    • Entomological Research
    • /
    • 제48권5호
    • /
    • pp.384-389
    • /
    • 2018
  • Aphis gossypii Glover is an important insect pest that functions as a viral vector and mediates approximately 45 different viral diseases. As part of a strategy for control of A. gossypii, we investigated the functions of genes using RNAi. To this end, a cDNA library was constructed for various genes and for selecting appropriate targets for RNAi mediated silencing. The cDNA library was constructed using the Gateway cloning system with site-specific recombination of bacteriophage ${\lambda}$. It was used to carry out single step cloning of A. gossypii cDNAs. As a result, a cDNA library with a titer of $8.4{\times}10^6$ was constructed. Since the sequences in this library carry att sites, they can be cloned into various binary vectors. This library will be of value for various studies. For later screening of selected genes, it is planned to clone the library into virus-induced gene silencing (VIGS) vectors, which makes it possible to analyze gene function and allow subsequent transfection of plants. Such transfection experiments will allow testing of RNAi-induced insecticidal activity or repellent activity to A. gossypii, and result in the identification of target genes. It is also expected that the constructed cDNA library will be useful for analysis of gene functions in A. gossypii.

EL/IX 단계 3을 적용한 실시간 운영체제 Qplus-P용 C 표준 라이브러리의 설계 및 구현 (The Design and Implementation of EL/LX level3 C Standard Library for RTOS Qplus-P)

  • 김도형;신창민;박승민
    • 정보처리학회논문지A
    • /
    • 제9A권4호
    • /
    • pp.485-490
    • /
    • 2002
  • 디지털 TV, 인터넷 셋탑박스, 인터넷 전화기 등과 같은 정보가전 제품이 속속 등장하면서 이들 제품의 기능을 제어하는데 필수적인 실시간 운영체제 시장이 크게 성장하고 있다. 한국전자통신연구원에서는 소형의 휴대 정보 단말에서부터 디지털 셋탑박스 및 홈 서버까지 다양한 종류의 정보가전 기기에 공통으로 사용될 수 있는 확장 가능한 표준 실시간 운영체제 Qplus-P를 개발하였다. 본 논문에서는 정보가전용 실시간 운영체제 Qplus-P에 탑재되는 C표준 라이브러리의 설계 및 구현에 대해 기술한다. Qplus-PC표준 라이브러리는 레드햇에서 실시간 운영체제 국제 표준으로 제안된 EL/LX 응용 프로그램 인터페이스 단계에 따라 설계되었다. 그리고 Qplus-P 응용 프로그램 수행에 필요한 Tiny-X, 카페 등을 지원하기 위해 추가적으로 필요한 함수들도 구현되었다. 구현된 C표준 라이브러리는 EL/IX 응용프로그램 인터페이스 단계를 적용하지 않은 C표준 라이브러리보다 라이브러리 크기를 30% 정도 줄일 수 있었다.

PUMA robot에서의 RCCL(robot control C library)의 구현 (Implemention of RCCL on PUMA)

  • 배본호;이진수
    • 제어로봇시스템학회:학술대회논문집
    • /
    • 제어로봇시스템학회 1991년도 한국자동제어학술회의논문집(국내학술편); KOEX, Seoul; 22-24 Oct. 1991
    • /
    • pp.24-29
    • /
    • 1991
  • RCCL(Robot Control C Library) is general purpose robot control language. It is programmed with C language and composed of C library. So it is well portable and supports sensor integration control and high level force control algorithms. We implemented RCCL on PUMA. We developed servo controller of DDC(Direct Digital Control). We used intel 8097BH one chip micro controller as CPU. One digital servo board controls three motors. Host computer is IBM PC 386DX-33 with RCCL.

  • PDF

누에 유충의 cDNA 유전자 은행 제작 및 cDNA 클론의 부분염기서울 분석 (Construction of the cDNA Library from Bombyx mori Larvae and Analysis of the Partial cDNA Sequences)

  • 김상현;윤은영
    • 한국잠사곤충학회지
    • /
    • 제38권1호
    • /
    • pp.13-18
    • /
    • 1996
  • 곤충의 다양한 기능해석을 유전자 수준에서 수행하기 위하여 주요 익충인 누에를 대상으로 유전 자원 확보를 시도하였다. 우선 5령의 누에유충에서 cDNA 유전자 은행을 제작하여 1.3 X 106개의 cDNA 유전자원을 확보하였다. 누에유충의 cDNA 유전자 은행에서 무작위로 plaques을 선정하였고, 이를 플라스미드로 전환하여 SK primer를 이용한 부분 염기서열을 결정하였다. 결정된 cDNA 클론의 부분 염기서열을 GenBank 데이타베이스에서 검색하여 37개의 발현 유전자 꼬리표를 생산하였다. 이들 중 15개는 데이터베이스와의 비교부위가 150bp 이상이고 DNA 상동성이 약 60% 이상으로 비교적 높은 DNA 상동 유의성을 나타내는 것으로 혈림프에서 발견되는 수종의 저장 단백질, 곤충의 기동성, 체벽 형성, 효소 및 초파리의 돌연변이 유전자형과 유사한 종류들이었다. 또한 15개의 발현 유전자 꼬리표 중 누에에서 밝혀진 것은 3종이고 그 나머지는 누에에서 처음 밝혀진 것으로 이 클론에 대한 정확한 동정이 요구된다.

  • PDF

C형 간염바이러스 E2 단백질에 결합하는 추정 세포수용체 cDNA의 클로닝 (Cloning of cDNA Encoding Putative Cellular Receptor Interacting with E2 protein of Hepatitis C Virus)

  • 이성락;백재은;석대현;박세광;최인학
    • 생명과학회지
    • /
    • 제13권4호
    • /
    • pp.541-550
    • /
    • 2003
  • 본 실험에서는 C형 간염바이러스 (HCV)의 외피 단백질인 E2 당단백질에 결합하는 세포단백질들을 클로닝하기 위해 간세포 cDNA를 phage 표면에 발현시킨 phage library를 제작하였고, 12-mer peptide library와 함께 E2 단백질에 대해 panning을 실시하였다. 검색결과 세포내 신호전달과 cytoskeleton 구성에 관여하는 tensin, membrane protein band 4.1 등 세포질내 단백질과 CCR7, CKR-L2, insulin-like growth factor-1 receptor 등 세포막 단백질 등이 확인되었다. 이들 단백질들을 발현하는 phage들은 수용성 E2단백질을 이용한 결합중화반응 결과 E2 단백질에 특이적으로 결합함이 확인되었다. 사람 T 세포에서 주로 발현되는 CCR7 유전자를 PHA로 활성화된 사람 T 세포의 total RNA를 이용하여 증폭하고 클로닝하였다. 293T 세포에 transfection시켜 단백질 발현양상을 flow cytometer로 분석하여 70% 이상의 세포들이 CCR7을 발현하고 있음을 관찰하였다. 수용성 E2 단백질을 CCR7이 transfection된 세포와 mock transfection된 대조군 세포에 각각 반응시킨 결과 dose-dependent 양상으로 CCR7에 결합하였다.

Construction of cDNA Library from Posterior Silk Gland (PSG) of Korean Oak Silkmoth, Antheraea yamamai and Molecular Cloning of Fibroin Heavy Chain Gene(FHC)

  • Lee, Jin-Sung;Kim, Soon-Jung;Kim, Ki-Hwan;Park, Young-Min;Suh, Dong-Sang
    • Journal of Life Science
    • /
    • 제10권1호
    • /
    • pp.10-13
    • /
    • 2000
  • To develope the genetic source of oak wild silkworm, Antheraea yamamai, the cDNA library was constructed with poly A+ mRNA isolated from posterial silk gland of fifth instar larvae. Titer of the cDNA library was about 5.1$\times$105 pfu in total. We presumed that the titer covered almost all transcripts existed in Antherea yamamai. From cDNA library of Antheraea yamamai, fibroin heavy chain gene, which is specifically expressed from posterial silk gland of Antheraea yamamai, was screened using oligonuclotide probe specific to alanine rich motif of fibrin heavy chain gene of Antheraea pernyi. As a result, fibroin clones isolated from 5$\times$104 plaques showed the highest homolgy (95%) with that of Antherea pernyi in nucleotide of Anthereaea yamamai and Bombyx mori shows that there is no homologous sequence in the 3+ partial 채야후 region Genomic southern hybridization suggested that one copy is present. Northern hybridization showed that fibroin transcript was approximateely 9 kb in length.