• 대한바이러스학회지
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• 제27권2호
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• pp.257-260
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• 1997

Adenoviruses are icosahedral virions containing double-stranded linea DNA. They are 70 nm to 90 nm in diameter and capsid is composed of 252 capsomeres. Several members of this group, including types commonly associated with respiratory disease in man, are capable of producing malignant tumors in young hamsters and a few types have been shown to be oncogenic in young rat. Previous report involving effect of caffein on transformation induced by Adenovirus type 12 [9] has been carried out. The present report represents a continuation of previous study. To obtain evidence concerning the effect of MNNG (N-methyl-N'-nitro-N-nitroguanidine) on transformation, investigation of adenovirus type 12 of this group was undertaken. For practical consideration it was desirable to investigate the effect of MNNG on the adenovirus type 12 induced transformation in L cell. Results were as following 1. Adeno virus type 12 induced transformation was enhanced in the presence of MNNG. 2. Yields of adeno type 12 virus in L cell were slightly inhibited by treatment of MNNG.

• Journal of Nutrition and Health
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• 제38권10호
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• pp.807-816
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• 2005

본 연구에서는 Sprague Dawley종 수컷 쥐에서 DHM로 대장암을 유발시킨 후 식이에 첨가한 n-3 RUFA 함량에 따라 대장의 암화과정에 어떤영향을 미치는지 생화학적인 기전을 검토하여 다음과 같은 결과를 얻었다. 1) 식이에 n-3 RUFA를 6.2 mmole 첨가하여 먹인 경우에는 COX-2의 mRNA와 단백질의 발현 및 TBX2와 PGE2 합성이 유의하게 감소 되었으며, 이에 따라 세포증식도 억제되었다. 그러나 n-3 RUFA를 12.4 mmole 첨가한 식이로 사육한 경우에는 오히려 COX-2의 mRNA와 단백질의 발현 및 $TXB_2$ 와 $PGE_2$ 합성이 대조군 보다도 더 많이 증가되었고 세포증식도 대조군과 같은 수준으로 증가하여 암화과정을 촉진하였다. 2) 식이에 n-3 PUFA를 6.2 mmole 첨가한 경우 대장 점막의 인지질의 지방산조성중 arachidonic 함량은 유의하게 낮았고, EPA와 DHA 함량은 유의하게 높았으며 n-3 PUFA를 12.4 mmole 첨가한 경우에는 EPA와 DHA 함량은 2배 이상 유의하게 더 높았다. 3) 대장 상피세포의 apoptosis는 식이에 n-3 PUFA를 첨가한 함량과는 관계없이 대조군에 비해 유의하게 약 34$\sim$$42\%$ 증가하였다. 4) 식이에 n-3 PUFA를 6.2 mmole 첨가하였을 때 Bax의 mRNA와 단백질 발현은 각각 유의하게 증가되었으나 n-3 PUFA를 12.4mmole 첨가한 경우에는 유의하게 감소되었다. 반면에Bcl-2의 mRNA와 단백질 발현은 n-3 PUFA 6.2 mmole 첨가한 경우에는 오히려 증가하였다. 총괄해서 본 연구결과에 의하면 항암효과가 있가도 알려진 n-3 PUFA는 식이에 첨가한 함량에 따라 암화과정에 미치는 효과가 다르게 나타났다, 그러므로 앞으로 대장의 암화과정을 억제시키는 n-3 PUFA의 적절량 또는 섭취의 한계치를 정하는 연구가 필요하다고 본다.

• 한국축산식품학회지
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• 제25권2호
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• pp.244-249
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• 2005

To investigate the effect of Holstein colostrum peptide fraction on proliferation of immune cell, polypeptide fractions were separated from acid whey into 3 fractions depending on molecular weight by ultrafiltration: Fraction I, which contains the polypeptide larger than 10,000 Da, Fraction n, which contains the polypeptide ranging from 1,000 Da to 10,000 Da and Fraction III, which contains the polypeptide smaller than 1,000 Da. EL-4 cell (murine T lymphoma cell) was used to evaluate immune enhancing effect of each fraction from Holstein colostrum. Fraction n showed the highest proliferative effect of the colostrum whey fractions on EL-4 cell at 1mg/mL compared with whole whey and other fractions and this proliferative activity was shown in dose dependent manner. Fraction n showed the highest proliferative effect on PMA (Phorbol 12-myristate 13-acetate) stimulated EL-4 cell. Heated Fraction n showed similar effect to native one on proliferation of both EL-4 cell and PMA stimulated EL-4 cell.

• 대한전자공학회논문지
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• 제22권3호
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• pp.1-5
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• 1985

Bridgnan방법으로 성장시킨 CuInse2단결정을 Se분위기 속에서 열처리하여 carrier농도가 2.6×1016/㎤인 n·Culnse2단결정을 얻었다. 이 단결정을 photoanode로 하고 polysulfide용액으로 3M KOH+3M Na2S+4M S를 사용하여 n·Culnsel-3M KOH+3M Na2S+4M S접합의 태양전지를 만들었다. 이 태양전지는 태양에너지 100mW/㎤의 조건하에서 FF=0.44이며, 태양에너지 변환효율은 5.67% 이었다.

• 한국컴퓨터산업학회논문지
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• 제6권5호
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• pp.757-766
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• 2005

There have been great demands for higher density SRAM in all area of SRAM applications, such as mobile, network, cache, and embedded applications. Therefore, aggressive shrinkage of 6T Full CMOS SRAM had been continued as the technology advances, However, conventional 6T Full CMOS SRAM has a basic limitation in the cell size because it needs 6 transistors on a silicon substrate compared to 1 transistor in a DRAM cell. The typical cell area of 6T Full CMOS SRAM is $70{\sim}90F^{2}$, which is too large compared to $8{\sim}9F^{2}$ of DRAM cell. With 80nm design rule using 193nm ArF lithography, the maximum density is 72M bits at the most. Therefore, pseudo SRAM or 1T SRAM, whose memory cell is the same as DRAM cell, is being adopted for the solution of the high density SRAM applications more than 64M bits. However, the refresh time limits not only the maximum operation temperature but also nearly all critical electrical characteristics of the products such as stand_by current and random access time. In order to overcome both the size penalty of the conventional 6T Full CMOS SRAM cell and the poor characteristics of the TFT load cell, we have developed $S^{3}$ cell. The Load pMOS and the Pass nMOS on ILD have nearly single crystal silicon channel according to the TEM and electron diffraction pattern analysis. In this study, we present $S^{3}$ SRAM cell technology with 100nm design rule in further detail, including the process integration and the basic characteristics of stacked single crystal silicon TFT.

• 한국전기전자재료학회논문지
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• 제19권4호
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• pp.314-321
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• 2006

There have been great demands for higher density SRAM in all area of SRAM applications, such as mobile, network, cache, and embedded applications. Therefore, aggressive shrinkage of 6 T Full CMOS SRAM had been continued as the technology advances. However, conventional 6 T Full CMOS SRAM has a basic limitation in the cell size because it needs 6 transistors on a silicon substrate compared to 1 transistor in a DRAM cell. The typical cell area of 6 T Full CMOS SRAM is $70{\sim}90\;F^2$, which is too large compared to $8{\sim}9\;F^2$ of DRAM cell. With 80 nm design rule using 193 nm ArF lithography, the maximum density is 72 Mbits at the most. Therefore, pseudo SRAM or 1 T SRAM, whose memory cell is the same as DRAM cell, is being adopted for the solution of the high density SRAM applications more than 64 M bits. However, the refresh time limits not only the maximum operation temperature but also nearly all critical electrical characteristics of the products such as stand_by current and random access time. In order to overcome both the size penalty of the conventional 6 T Full CMOS SRAM cell and the poor characteristics of the TFT load cell, we have developed S3 cell. The Load pMOS and the Pass nMOS on ILD have nearly single crystal silicon channel according to the TEM and electron diffraction pattern analysis. In this study, we present $S^3$ SRAM cell technology with 100 nm design rule in further detail, including the process integration and the basic characteristics of stacked single crystal silicon TFT.

• Tuberculosis and Respiratory Diseases
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• 제40권6호
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• pp.659-668
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• 1993

연구배경 : p53은 흔히 종양 억제 유전자로 생각되며, 그것의 변화는 비소세포 폐암을 포함하는 여러 악성 종양에 관여하게 된다. 그런, p53 발현율은 저자들의 보고마다 그리고 서로 다른 세포형에서 차이가 있다. 또한, p53의 발견시기가 조기인지 또는 후기인지도 명확치 않다. 이에, 저자들은 서로 다른 세포형과 조직에서의 p53 발현율을 조사하기 위해 그리고, 조기 또는 후기의 어느 시기에 발현하는지를 알아보기 위해 본 연구를 시작하였다. 방법 : 비소세포 폐암환자 50명으로부터 얻은 71개의 조직을 대상으로 비특이적인 단일클론 항체를 이용한 비교적 간단한 면역조직화학적염색을 시행하였다. 결과: 1) 비소세포 폐암환자에서 폐조직에서의 전체적인 p53 발현율은 46.5%(20/43)로 림프절의 25.0%(6/24)에 비해 높았으나, 통계적인 유의성은 없었다. 2) 세포형에 따른 폐조직에서의 p53 발현용은 편평세포암과 선암에서 각각 58.3%와 50.0%로 두 군간의 유의한 차이는 없었다. 3) 병기에 따른 폐조직에서의 p53 발현율은 I기, II기, IIIA기, IIIB기 및 IV기 각각에서 33.3%, 60.0%, 40.0%, 60.0%, 66.7% 이었으며, 병기에 따른 발현율의 유의한 차이는 없었다. 또한, 낮은 병기(I기 및 II기)와 진행된 병기(IIIa기, IIIb기 및 IV기)간에도 유의한 차이는 없었다. 4) T 지표에 따른 p53 발현율은 T1, T2, T3 및 T4에서 각각 33.3%, 50.0%, 16.7% 및 100%로 T4에서 발현율이 높았으나 대상 환자수가 적어 의의를 둘 수가 없었다. N 지표에 따른 발현율은 N1, N2 및 N3에서 각각 27.2%, 22.2% 및 25.0%로 발현율의 유의한 차이는 없었다. 5) 폐조직에서 양성반응을 보이고 림프절 침범이 있었던 7명의 환자들에서 N1, N2의 발현율은 각각 12.5%(1/8)과 50.0%(2/4)이었다. 6) 폐조직에서 음성반응을 보이고 림프절 침범이 있었던 5명의 환자들에서 발현되는 림프절은 없었다. 결론 : 이상의 결과로 비소세포 폐암에서의 p53 발현율은 세포형과 병기의 진행과는 관련이 없는 것으로 생각되며, 폐암 발생 및 진행의 어느 시기에 관여하는지에 대해서는 또 다른 연구가 필요하리라 생각되었다.

• 한국환경농학회지
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• 제23권4호
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• pp.228-233
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• 2004

Nitrate removal was examined from May to October 2003 of a surface flow treatment wetland cell, which was a part of a treatment wetland system composed of four wetland cells and a distribution pond The system was established on rice paddy near the Kohung Estuarine Lake located in the southern part of the Korean Peninsula. Effluent from a secondary-level night soil treatment plant was funneled into the system. The investigated cell, 87 m in length and 14 m in width, was created in April 2003. An open water was designed at its center, which was equivalent to 10 percent of its total area. Cattails (Typha angustifolia) were transplanted from natural wetlands into the cell and their stems were cut at about 40cm height from their bottom ends. Average $25.0\;m^3/day$ of effluent from the treatment plant was funneled into the cell by gravity flow and average $24.1\;m^3/day$ of its treated effluent was discharged into the Sinyang Stream flowing into the lake. Its water depth was maintained about 0.2 m and its hydraulic detention time averaged 5.2 days. Average height of the cattail stems was 42.5 cm in May 2M3 and 117.7 cm in September 2003. The number of stems averaged $9.5\;stems/m^2$ in May 2003 and $16.4\;stems/m^2$ in September 2003. The growth of cattails was good. Temperature of influent and effluent averaged 25.9 and $26.7^{\circ}C$, respectively. $NO_3$-N loading rate of influent and effluent averaged 176.67 and $88.09\;mg/m^2\;day$, respectively. Removal of rf03-N averaged $89.58\;mg/m^2\;day$ and its removal rate by mass was about 50%. Considering its initial operating stage in which cattail rhizomes and litter layer on the bottom were not Idly established, the $NO_3$-N removal rate of the cell was rather good.

• Molecules and Cells
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• 제24권3호
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• pp.416-423
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• 2007

Alterations in the glycan chains of cell surface glycoconjugates are frequently involved biological processes such as cell-cell interaction, cell migration, differentiation and development. Cultured embryonic (E18) rat cortical neurons underwent apoptosis in response to camptothecin, and lectin histochemistry showed that binding to apoptotic neurons of FITC-conjugated Maackia amurensis agglutinin (MAA), which is specific for terminal ${\alpha}2,3$-sialic acid residues, increased progressively with increasing concentrations of camptothecin. Analysis of the total proteins of apoptotic neurons by SDS-PAGE, and lectin blotting using HRP-labeled MAA, revealed that the expression of terminal ${\alpha}2,3$-sialic acid residues on an unknown protein with an apparent molecular mass of 25.6 kDa also increased in apoptotic neurons. NP-HPLC analysis of the total cellular N-glycans of normal and apoptotic neurons demonstrated that the expression of structurally simpler biantennary types of N-glycans fell by 49% during apoptosis whereas the more branched triantennary types of N-glycans with terminal sialic acid residues increased by up to 59%. These results suggest that increased surface expression of ${\alpha}2,3$-sialic acid residues and hyperglycosylation of N-glycans is a common feature of cellular responses to changes in cell physiology such as tumorigenesis and apoptosis.

• 대한미생물학회지
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• 제22권2호
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• pp.167-174
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• 1987

N-myc, a DNA sequence related to the oncogene c-myc, was found to be amplified in untreated primary neuroblastomas and the amplification appeared to be associated with advanced disease at diagnosis and rapid tumor progression. Synthetic peptides have been useful immunogens for generating antisera and monoclonal antibodies to a number of native proteins. In order to identify myc-related protein in the tumor cells, an antiserum against a synthetic hexapeptide (-Glu-Asp-Ile-Trp-Lys-Lys-), whose sequence corresponds to a part of the exon 2 of oncogene N-myc, was prepared by immunizing a rabbit with BSA-conjugated peptide. After ammonium sulfate precipitation and affinity column chromatography, it appeared to be specific to the peptide. Strong nuclear staining in immunoperoxidase method using this serum was observed in both human promyeloid leukemic cell line, HL-60(containing high c-myc copy number), and human neuroblastoma cell line, LA-N-5 (containing high N-myc copy number), whereas LA351 (human lymphoid cell line) cells did not react with the serum. This reaction was completely abrogated by incubating the antiserum with soluble excess peptide. These data suggest that the protein encoded by N-myc could be localized in the nucleus as c-myc protein and this antiserum can be used to detect myc-related tumor cells in clinical samples and to determine if the N-myc expression correlates with genomic amplification in cell lines, untreated primary tumors, and untreated metastases.