Translationally controlled tumor protein (TCTP) is one of important immune regulator. TCTP has been implicated in cellular processes including the cell growth, cell cycle progression, apoptosis regulation and the protection of cells against various stress condition. In this study, we cloned and characterized TCTP from rock bream (Oplegnathus fasciatus), which is an economically important species in the Korea aquaculture industry. The Full-length of rock bream TCTP (RbTCTP) cDNA was 1041 bp and contained an open reading frame (ORF) of 513 bp, which encoded 170 amino acid sequence. The 5' untranslated region (UTR) was 90 bp while the 3' UTR was 538 bp, containing a polyadenylation signal (ATTAAA). The identity of amino acid sequence was 76%, 75% and 74% in tilapia, orange-spotted grouper and Japanese seaperch, respectively. The positions of microtuble-binding region, Ca⁺ binding region and TCTP signature regions in RbTCTP were similar with those of other fish species and mammalian. The RbTCTP mRNA was expressed highest in the muscle. Expression of TCTP mRNA were significantly variable according to injection of red seabream iridovirus (RSIV), Streptococcosis (S. iniae) and Edwardsiella tarda (E. tarda).

The molecular responses to various abiotic stresses were investigated by the approaches with transcriptomic analysis based on an ACP system. Here we identified differentially expressed genes under abiotic stresses in alfalfa seedlings and they were mostly unknown genes and a few common stress-related genes. Among them, mitochondrial small HSP23 was responded by the diverse stress treatment such as heat, salt, As stresses and thus it could be a strong candidate that may confer the abiotic stress tolerance to plants. When expressed in bacteria, recombinant MsHSP23 conferred tolerance to salinity and arsenic stress. Furthermore, MsHSP23 was cloned in a plant expressing vector and transformed into tobacco, a eukaryotic model organism. The transgenic plants exhibited enhanced tolerance to salinity and arsenic stress under ex vitro conditions. In comparison to wild type plants, the transgenic plants exhibited significantly lower electrolyte leakage. Moreover, the transgenic plants had superior germination rates when placed on medium containing arsenic. Taken together, these overexpression results imply that MsHSP23 plays an important role in salinity and arsenic stress tolerance in transgenic tobacco. The results of the present study show that overexpression of alfalfa mitochondrial MsHSP23 in both eukaryotic and prokaryotic model systems confers enhanced tolerance to salt and arsenic stress. This indicates that MsHSP23 could be used potentially for the development of stress tolerant transgenic crops, such as forages.

Liriope platyphylla has been though as an useful medical plant to improve the cough, sputum, neurodegenerative disorders, obesity, and diabetes in Korea and China from old times. In order to investigate the effects of Liriope platyphylla on expression and secretion of nerve growth factor (NGF), the mRNA expression and protein secretion were detected in the neuronal cell (B35) and neuroglial cell (C6) cultured with three differences concentration (5%, 10%, 15%) of Liriope platyphylla. In MTT assay and FACS anslysis, the some death of some B35 and C6 cells were observed in 15% extract-treated group, while other groups did not induce the death. Also, the mRNA expression of NGF were significantly increased in 5% and 10% extracts treated-group. Furthermore, the NGF protein concentration in supernatant collected from cultured cells showed the very similar pattern with mRNA expression. In order to verify the activity of secreted NGF, the culture supernatant collected from B35 and C6 cells cultured with Liriope platyphylla extracts for 24 hrs were treated into undifferentiated PC12 cells, and the differentiation level of PC12 cell were also observed with microscopes. The differentiation level of PC12 cell were significantly increased depend on the dose of extract. Therefore, these results suggested that the water extracts of Liriope platyphylla may contribute the regulation of NGF expression and secretion in the neuronal cell and be considered as an excellent candidate for a neurodegenerative disease-therapeutic drug.

Pectin, one of the main components of plant cell wall, is deesterified in muro by PME (Pectin methylesterase). PME activity is particularly regulated by inhibitor proteins known as the pectin methylesterase inhibitor (PMEI). The PMEI plays a key role in wounding, osmotic stress, senescence and seed development. However, the role of PMEI in plant species still remains to be demonstrated especially in wheat. To facilitate the studies on the expression of the TaPMEI gene, RT-PCR was performed using leaf, stem and root tissues in response to exogeneous application of phytohormones and abiotic stress treatments. Transcription of the TaPMEI gene was significantly induced in NaCl, H2O2 and SA treatments, and reduced when plants were treated with ABA. To elucidate the subcellular localization of the TaPMEI protein, TaPMEI:GFP fusion construct was transformed into onion epidermal cells by particle bombardment. The fluorescence signal was exclusively detected in cell wall of the cells. In order to obtain recombinant TaPMEI protein, the TaPMEI protein, expressed in E.coli as a MBP (~42.5 kDa) fusion protein recombinant. Purification and functinal analysis of TaPMEI as an inhibitor of PME activity are described.

Rice as a typical silicified plants needs the intemal absorption of silica, especially during the growing period. The leaves and culm of plant are erected up by uptake of silicic acid. Sun light could reach the bottom leaves in the plant communities. In addition, the nitrogen uptake would be physiologically controlled by the application of silica and the quality of rice could be improved by reducing the quantity of protein in grian. In the field experiment designed, the rice cultivar was DonhjinⅠho, Daeanbyeo and transplanting day was May 25, 2007. N levels per ha were 100 and 200kg, respectively and liquid silica(ai 11%, manufactureed by Dongbuhiteck Co.) was sprayed on flag leaves according to 500fold and 1000fold with distilled water and 3 times at an interval of 1week from 30 days before heading. The rice culms treated with each liquid silica levels were shortened and panicle length were increase as compare with the control in the level of each N. The lodging was reduced in the plot that treated with the higher liquid silica application of 100kg as compared with 200kg plot in the filed. The rice yields of the plots treated with silica application were more increased than in the control plot. All yield components, except of panicle number in DongjinⅠ, increased as compare with 200kg plot in the filed. Changes measured by 2-DE in display expression of flag leaves and seed in relation to nitrogen treatment level and silica trements were similar in fashion, yet still displayed distinguishable differences in display strength spots.

Recently with increase tendency of direct sowing cultivation, lodging problem which affect to the high quality rice plant is again raising its ahead. In order to reduce this lodging problem there is a chemical method which uses plant growth retardant. This experiment was conducted to evaluate the effect of lodging reduction as affected by plant growth retardant which is IBP-Metconazole (IPM) in direct-seeded rice on flooded paddy field. IPM treatment carried out 50, 40, 30 days before heading. Hexaconazole treatment carried out 30 days before heading. IPM treatment 30 days before heading resulted the shortest plant culm among the IPM treatments. 4 internode length was shorter by 3.75㎝ in IPM treatmenst than in control. breaking strength was not a difference from between IPM treatments but breaking strength was significantly increased by IPM treatments than control. IPM treatments increased yield 10~11% as compared with control. The protein contents of flag leaves by 2-DE were visually higher in the plot treated with the IPM application than in the plot control plot. The proteome approach to elucidate the mechanism which inhibited gibberellin synthase will be future performed in the on-going research.

We have cloned an LTP gene (PoLTP1) from poplar (Populus alba × P. tremula var. glandulosa) suspension cells and examined changes in its expression levels in response to various stresses and ABA treatment. The full-length PoLTP1 cDNA clone encodes a polypeptide of 116 amino acids with typical characteristics of LTPs, notably a conserved arrangement of cysteine residues. Southern blot analysis indicate that two or three copies of the PoLTP1 are present in the genome of the investigated hybrid poplar. In addition, northern analysis of samples from soil-grown plants indicate that PoLTP1 is tissue-specifically expressed in the leaves and flowers. The gene is significantly up-regulated by treatment with mannitol, NaCl and ABA, but not by either cold or wounding. These results indicate that PoLTP1 is involved in osmotic stress responses in poplar plants and suspension cells.

레티놀 결합 단백질(retinol-binding protein, RBP)은 고등 척추동물에서 혈류를 통해 특이적으로 레티놀을 표적세포에 운반해 주는 중요한 역할을 한다. 우리나라의 연안에 서식하고 있으며 산업적으로 중요한 조피볼락(Sebastes schlegeli)을 대상으로 4-nonylphenol(NP)가 RBP mRNA 발현에 미치는 영향을 구명하기 위해 간으로부터 cDNA library를 제작하고 RBP 단편의 염기서열을 분석하였다. 분석된 RB

더덕의 뿌리로부터 aluminum스트레스와 관련이 있는 aluminum induce protein(ClAIP)유전자를 분리하였다. ClAIP 유전자의 염기서열를 분석한 결과 906 bp 길이로, 236개의 아미노산으로 번역되는 711bp의 ORF를 가지고 있으며, A. marina(84%), G. hirsutum(84%), V. radiata(83%), A. thaliana(80%), B. hapus(78%), T. aestivum(68%) 등 다른 식물에서 밝혀져 있는 aluminum induce protein과 높은 상동성을 나타내었고, N-terminal에는 Asn synthetase영역이 존재하고 있다. 더덕에서 분리한 aluminum induced protein(ClAIP)을 aluminum처리 농도와 시간에 따른 ClAIP유전자의 발현양상을 알아보고자 50uM Al3+ 를 처리 후 시간대별로 RT-PCR을 수행한 결과 시간이 지남에 따라 ClAIP유전자의 발현이 증가되는 것으로 나타났다 중금속, 염 , 온도에 대한 유전자의 발현양상을 조사하기 위 해 50uM CdCl,2, 20 uM CuSO4, 50uM Fe2O3, 100 uM NaCl를 2일과 42℃에서 4시간 처리 후 발현량을 조사한 결과 카드뮴(Cd)에 대해서 특이적으로 반응하는 것으로 나타났다.

We tried to introduce two forsythia genes related in lignan biosynthesis, dirigent protein and pinoresinol/lariciresinol (Ph) reductase, into potatoes for accumulation of lignans in transgenic potatoes. We made binary vectors overexpressing dirigent protein gene and P/L reductase gene driven by a CaMV35S promoter and transformed into potatoes via Agrobacterium mediated transformation. And in order to control the metabolic flux of lignan biosynthesis pathway, we tried to inhibit chalcone synthase genes of potatoes by antisense inhibition technique also. We tried to use PCR screening method for selection of transgenic plants of different vectors. We tried to determine and compare lignan contents from different transgenic potato lines.