1.Nucleotide sequence analysis of Maaji viral cDNA amplified by Hantaan virus specific primers.
Pyung Woo LEE ; Dong Hoon CHUNG
Journal of the Korean Society of Virology 1993;23(1):57-67
No abstract available.
Base Sequence*
;
DNA, Complementary*
;
Hantaan virus*
2.Identification of Matrix Mineralization-Related Genes in Human Periodontal Ligament Cells Using cDNA Microarray.
Jae Hee SHIN ; Jin Woo PARK ; Shin Il YEO ; Woo Chang NOH ; Moon Kyu KIM ; Jung Chul KIM ; Jo Young SUH
The Journal of the Korean Academy of Periodontology 2007;37(Suppl):447-463
No abstract available.
Apoptosis
;
DNA, Complementary*
;
Humans*
;
Oligonucleotide Array Sequence Analysis*
;
Periodontal Ligament*
3.An Iterative Normalization Algorithm for cDNA Microarray Medical Data Analysis.
Yoonhee KIM ; Woong Yang PARK ; Ho KIM
Genomics & Informatics 2004;2(2):92-98
No Abstract available.
DNA, Complementary*
;
Oligonucleotide Array Sequence Analysis*
;
Statistics as Topic*
5.Cloning and expression analysis in resurrection process of trehalose-6-phosphate synthase gene from Selaginella tamariscina.
Cai-Cai XI ; Wei GU ; Hong-Mei SUN ; Rong TIAN ; Qi LIU ; Xiao-Hao WANG
China Journal of Chinese Materia Medica 2018;43(24):4842-4849
Selaginella tamariscina is a typical resuscitation medicinal plant with extreme drought tolerance. Trehalose plays an important role in the resurrection process, and the trehalose-6-phosphate synthase(TPS) is the key enzyme to synthesize trehalose in plants. In this study, the sequence of TPS was obtained by splicing from the transcriptome data of S. tamariscina. After the synthesis of cDNA based on the template of total RNA, the sequence was cloned by RT-PCR for verification and then analyzed by bioinformatics methods. The results indicated that the full-length coding sequence of StTPS was 2 799 bp (GenBank accession no. MH155231), and the encoded protein contained 932 amino acids. StTPS could be located in the chloroplastid according to subcellular localization prediction. There were two conserved domains belonging to glycogen phosphorylase glycosyltransferase (GPGTF) family but no signal peptide or transmembrane domain in StTPS. The expression of StTPS was determined by qRT-PCR and the variation of trehalose content was measured by HPLC-ELSD during the resurrection process of S. tamariscina. Meanwhile, the correlation between them was analyzed. The results showed that both the expression level of StTPS and the trehalose content increased associated with the extension of dehydration time, and declined associated with the extension of rehydration time which proved a significant positive correlation between the StTPS expression level and the trehalose content. The results suggested that the StTPS probably plays a central role in recovery process in S. tamariscina.
Amino Acid Sequence
;
DNA, Complementary
;
Glucosyltransferases
;
Selaginellaceae
;
Trehalose
6.Role of STAT3-Interacting Protein (STIP1) in delta12-Prostaglandin J2-Induced Cell Death.
Seong Mook KIM ; Sun LEE ; Hwan Jong KWAK ; Bo Eun KIM ; Dong Jin KIM ; In Kyung KIM ; Seong Whan JEONG
The Korean Journal of Physiology and Pharmacology 2004;8(1):27-31
delta12-Prostaglandin J2 (delta12-PGJ2) is one of cyclopentenone prostaglandins. The delta12-PGJ2 is known to induce apoptosis of tumor cells, however, it's action mechanism is not clear. It has recently been reported that STAT3 is involved in tumorigenesis. In the present study, we investigated the role of STAT3-interacting protein (STIP1) in the cytotoxicity of delta12-PGJ2, since STIP1 was recently reported as a modulator of STAT3 activation by specifically binding to inactive (unphosphorylated) STAT3. The effect of delta12-PGJ2 was observed in stably overexpressing Neuro-2A cells transfected with full cDNA of STIP1, and cytotoxicity of delta12-PGJ2 in the transfected cells was increased, compared with the vector control cells. The cytotoxicity of delta12-PGJ2 treatment was significantly accentuated by pretreatment of the STIP1-transfected cells with protein kinase inhibitor, genistein, and less activation of STAT3 in STIP1-transfected cells was shown, compared with the vector control cells. Expression of bax was also increased in the STIP1-transfected cells. These data suggest that STIP1 inhibits cell growth via inhibition of STAT3 activation in delta12-PGJ2 treatment.
Apoptosis
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Carcinogenesis
;
Cell Death*
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DNA, Complementary
;
Genistein
;
Prostaglandins
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Protein Kinases
7.Biochemical and Genetic Analysis of Seven Korean Individuals With Suspected Metachromatic Leukodystrophy.
Minje HAN ; Sun Hee JUN ; Yun Jin LEE ; Baik Lin EUN ; Seung Jun LEE ; Moon Woo SEONG ; Sung Sup PARK ; Sang Hoon SONG ; Hyung Doo PARK ; Junghan SONG
Annals of Laboratory Medicine 2015;35(4):458-462
Metachromatic leukodystrophy (MLD) is an autosomal recessive disease caused by a deficiency in arylsulfatase A (ARSA). However, decreased ARSA activity is also observed in pseudodeficiency (PD). To distinguish between MLD and PD, we performed gene mutation and sulfatide analyses by using dried blood spots (DBSs) from seven Korean individuals who underwent an analysis of ARSA activity. DNA was extracted from DBSs, and PCR-direct sequencing of ARSA was performed. The cDNA obtained was analyzed to confirm a novel mutation. Of the seven subjects, three were confirmed as having MLD, one was confirmed as having MLD-PD, one was confirmed as having PD, and the remaining two were obligate heterozygotes. We verified the novel pathogenic variant c.1107+1delG by performing familial and cDNA analyses. Sulfatide concentrations in DBSs were analyzed and were quantified by using ultra-performance liquid chromatography and tandem mass spectrometry, respectively. Total sulfatide concentration was inversely correlated with ARSA activity (Spearman's coefficient of rank correlation, P=0.929, P=0.0025). The results of this mutational and biochemical study on MLD will increase our understanding of the genetic characteristics of MLD in Koreans.
Cerebroside-Sulfatase
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Chromatography, Liquid
;
DNA
;
DNA, Complementary
;
Heterozygote
;
Leukodystrophy, Metachromatic*
;
Tandem Mass Spectrometry
8.Several Genes Expressed During Morphogenesis of Lentinus edodes (ImHyup-1).
Sang Sun LEE ; Sung Woon HONG ; Seung Hae KIM ; Bong Cheol KIM
Mycobiology 2001;29(3):135-141
Differential display of reverse transcription (DDRT)-PCR was conducted to have a profile of the differentially expressed genes during the formation of fruiting body of Lentinus edodes. The lines of L. edodes (ImHyup-1) employed were cultivated in the artificial blocks of sawdust, and the fruiting body was induced from the mycelia or the mass protruded from the brown surface of the sawdust blocks. RNAs were prepared from the four different developmental stages; mycelial, primordial, and stipes and pileus of fruiting body. The fragments of cDNA were synthesized from the combinations of the arbitrary primers and 3' one anchored Oligo-dT primer. Twelve combinations using the primers have been tested, and among them nineteen bands were identified as differentially expressed. Those genes were further analyzed by DNA sequencing and followed by homology search. Characterization of one clone was conducted as a preliminary data and more are under investigation.
Clone Cells
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DNA, Complementary
;
Fruit
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Lentinula*
;
Morphogenesis*
;
Reverse Transcription
;
RNA
;
Sequence Analysis, DNA
;
Shiitake Mushrooms*
9.Renal Adaptive Responses of Na+-K+-APTase Subunit Isoforms to Chronic Hypokalemia.
Kyu Youn AHN ; Sug Chae KIM ; Bum MOON ; Kyung Keun KIM ; Baik Yoon KIM
Korean Journal of Anatomy 1998;31(3):405-418
Chronic hypokalemia alters Na+-K+-ATPase gene expression in several tissues. While it is established that Na+-K+-ATPase activity and alpha1 and beta1 subunit protein levels increase during K depletion in the outer medullary collecting duct (OMCD) and do not significantly change in the cortical collecting duct (CCD), little is known about the adaptive responses of the other isoforms in these other nephron segments. Accordingly, this study was performed to characterize the relative levels of expression and cellular distribution of mRNAs encoding the Na+-K+-ATPase subunit isoforms in normal and K-deprived (2 weeks) rats using the Northern analysis and in situ hybridization (ISH). Isoform specific 32P-labeled cDNA (for Northerns) or digoxigenin labeled cRNA (for ISH) probes were used. In normal rats, the order of expression amounts of all isoforms mRNAs from highest was outer medulla > cortex > inner medulla, and that of K-deprived rats was outer medulla > inner medulla > cortex. alpha1 mRNA levels were much greater than those of alpha2 or alpha3 in cortex, outer and inner medulla. mRNA levels for all isoforms were 2~3 folds greater in inner medulla of K-deprived rats compared to controls. In contrasts, the levels of all isoforms mRNAs in cortex and outer medulla were comparable between the two gruops. By ISH, mRNAs for all isoforms were observed in the S3 segment of proximal tubule, the cortical thick ascending limb (CTAL), medullary thick ascending limb (MTAL), distal convoluted tubule (DCT), connecting tuble (CNT), and the entire collecting duct. Both groups exhibited comparable cellular patterns of labeling, but the signal intensity of K-deprived rats was much greater in the proximal portion of the inner stripe of outer medullary collecting duct (OMCDi) and proximal portion of the inner medullary collecting duct (IMCD), and less in the MTAL compared to controls. The signal intensity of alpha1, alpha3, and beta1 isoforms was less in the CTAL, DCT, and CCD of K-deprived rats, but alpha2 isoform was slightly increased. These results suggest that chronic hypokalemia enhances expression of Na+-K+-ATPase subunit isoforms in the proximal portion of OMCDi and proximal IMCD, but not other nephron segments, and that these isoforms may participate in potassium conservation by these segments during potassium deprivation.
Animals
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Digoxigenin
;
DNA, Complementary
;
Extremities
;
Gene Expression
;
Hypokalemia*
;
In Situ Hybridization
;
Kidney
;
Nephrons
;
Potassium
;
Protein Isoforms*
;
Rats
;
RNA, Complementary
;
RNA, Messenger
10.Modification of pGH cDNA using the first intron and adenovirus-mediated expression in CHO cells.
Xiujin LI ; Fei ZHONG ; Shunzhang QI
Chinese Medical Journal 2003;116(8):1267-1269
OBJECTIVEThis study was conducted to investigate the function of the first intron of porcine growth hormone (pGH) gene in the gene expression.
METHODSPCR method was used to amplify the first intron from pig genomic DNA. The intron was then inserted into pGH cDNA to construct pGH cDNA-intron (pGH cDNA-in). The recombinant adenoviruses containing pGH cDNA and pGH cDNA-in genes under control of CMV promoter were generated by homologous recombination method in HEK 293 cells respectively. The effect of the first intron on gene expression was evaluated by comparing the expression levels of pGH cDNA-in and pGH cDNA mediated by adenovirus vectors in CHO cells.
RESULTSThe expression level of pGH cDNA containing the first intron increased by 117%, which was significantly higher than that of pGH cDNA without the intron (P < 0.001).
CONCLUSIONThe first intron of pGH gene has the function to improve pGH gene expression.
Adenoviridae ; genetics ; Animals ; CHO Cells ; Cricetinae ; DNA Transposable Elements ; DNA, Complementary ; DNA, Recombinant ; Genetic Vectors ; Growth Hormone ; genetics ; Introns ; Swine