• 한국동물학회지
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• 제39권3호
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• pp.292-298
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• 1996

안점의 꽃갯지렁이(Pseudopotamilla occelata)의 난자형성중 난황단백질의 전구체인 체강액 단백질(CP)은 수용체에 의해 중개되는데 이러한 수용체 중개에 의한 난모세포내로의 유입은 GTP-binding protein에 의해 조절되는 것으로 확인되었다. 체강액 단백질(CP)을 가장 활발히 투과시키는 중기 난모세포내로의 125 I-CP의 유입은 GTP에 의해 촉지되었고, GTP 유사체인 GTPrS나 GTP$\beta$S의 효과를 금입자로 표지된 체강액 단백질을 이용하여 전자현미경으로 확인해 본 결과, gold-labeled CP는 난황립에 집중되었고, 이러한 현상도 GTP에 의해서는 촉진되었고 GTPrS에 의해서는 억제되었다.

• Journal of Plant Biology
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• 제33권3호
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• pp.211-215
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• 1990

There is a family of homologous proteins known to small GTP-inding proteins which have a GTP binding domains and GTPase activity with molecular weight of about 20000 in mammalian tissues. Recently at least 20 different small GTP-binding proteins including three rasproto-oncogene, smg25, rho, and ral gene products were identified. These proteins play a central role in cellular prolifration, neoplasia, signal transduction, terminal differentiation, and secretory process of the cells. In this review, I have briefly compiled current information on the different areas of research in the small GTP-binding proteins in an attempt to convey an overall view of the fundamental role that this family of protein in normal cellular processes. Moreover, furture goals of research in the small GTP-binding proteins as well as the possible existence of this family of proteins in plant cells were discussed.

• Journal of Plant Biology
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• 제39권2호
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• pp.85-92
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• 1996

Small GTP-binding proteins are divided into three major group: Ras, Rho and Ypt/Rab. They have the conserved regions designed G1 to G5 that are critical in GDP/GTP exchange, GTP-induced conformational change and GTP hydrolysis. We isolated and characterized genomic DNA or cDNAfragments encoding G1 to G3 domains of small GTP-binding protein Rab and Rho from several plant species using two different PCR-based cloning strategies. Seven rab DNA fragments were isolated from 4 different plants, mung-bean, tobacco, rice and pepper using two degenerate primers corresponding to the GTP-binding domain G1 and G3 in small GTP-binding proteins. The amino acid sequences among these rab DNA fragments and other known small GTP-binding proteins shows that they belong to the Ypt/Rab family. Six rho DNA fragments were isolated from 5 different plants, mung-bean, rice, Arabidopsis, Allium and Gonyaulax using the nested PCR method that involves four degenerate primers corresponding to the GTP-binding domain G1, G3 and G4. The rho DNA fragments cloned show more than 90% homology to each other. Sequence comparison between plant and other known Rho family genes suggests that they are closely related (67 to 82% amino acid identity). Sequence analysis and southern blot analysis of rab and rho in mung-bean suggest than thses genes are encoded by multigene family in mung-bean.

• 한국식물병리학회:학술대회논문집
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• 한국식물병리학회 2003년도 정기총회 및 추계학술발표회
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• pp.81.2-82
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• 2003

Plants have evolved along with pathogens, and they have developed sophisticated defense systems against specific microorganisms to survive. G-protons are considered one of the upstream signaling components working as a key for the defense signal transduction pathway. For activation and inactivation of G-protein, GTP-biding proteins are involved. GTP -binding proteins are found in all organisms. Small GTP-binding proteins, having masses of 21 to 30kD, belong to a superfamily, often named the Ras supefamily because the founding members are encoded by human Ras genes initially discovered as cellular homologs of the viral ras oncogene. Members of this supefamily share several common structural features, including several guanine nucleotide binding domains and an effector binding domain. However, exhibiting a remarkable diversity in both structure and function. They are important molecular switches that cycle between the GDP-bound inactive form into the GTP-bound active form through GDP/GTP replacement. In addition, most GTP-binding proteins cycle between membrane-bound and cytosolic forms. such as the RAC family are cytosolic signal transduction proteins that often are involved in processing of extracellular stimuli. Plant RAC proteins are implicated in regulation of plant cell architecture secondary wall formation, meristem signaling, and defense against pathogens. But their molecular mechanisms and functions are not well known. We isolated a RacB homolog from rice to study its role of defense against pathogens. We introduced the constitutively active and the dominant negative forms of the GTP-hinging protein OsRacB into the wild type rice. The dominant negative foms are using two forms (full-sequence and specific RNA interference with RacB). Employing southern, and protein analysis, we examine to different things between the wild type and the transformed plant. And analyzing biolistic bombardment of onion epidermal cell with GFP-RacB fusion protein revealed association with the nucle.

• 한국동물학회지
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• 제37권1호
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• pp.40-48
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• 1994

세포분화에 따른 Small GTP-binding protein의 역할을 밝히기 위하여 Retinoic acid(RA)와 dibutyryl cyclic AMP(dbcAMP)로 분화를 유도한 F9 기형암종세포의 형태적인 변화와 함께 Small GTP-binding protein의 분포를 조사하였다. RA와 dbcAMP를 처리한 세포는 분화유도 5일경(초기 분화 단계)에 분명한 세포의 경계를 보이기 시작하여 7일경(분화 후기 단계)에는 거의 모든 세포가 등근 분화된 형태로 전환되었다. 이 분화과정 동안 세포막에는 많은 microvilli와 lamellopodia 같은 구조물이 나타났다. 아울러 초기 분화 단계에 많은 량의 laminin이 발현되었으며 분화 후기에 microtubule의 재분포가 관찰되었다. 세종류의 Small GTP-binding protein(25 23, 21 KD)이 F9 세포의 막성분과 세포질에서 관찰되었으며 분화가 진행됨에 따라서 세단백질 모두 증가되는 양상을 보였다 이러한 결과는 Small GTP-binding protein이 F9 세포의 분화에 특별한 기능을 가지고 있음을 시사해 주고 있다.

• Journal of Yeungnam Medical Science
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• 제10권2호
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• pp.360-368
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• 1993

세포막 정보전달 경로에서 수용체에 전달된 정보를 세포내로 전달하는데 조절 단백질로 알려진 GTP 결합단백질을 소외 뇌조직으로부터 정제하고 그 분자량등을 관찰하였다. 분쇄한 소의 뇌조직으로부터 세포막을 분리 해내고 1% cholate를 이용하여 세포막 단백질을 얻었으며 DEAE-Sephacel column chromatography를 시행하였다. 여기서 얻은 GTP 결합단백질은 다시 Ultrogel AcA 34 column chromatography, heptylamine-Sepharose column chromatography 순으로 실시하여 $GTP{\gamma}S$와 결합하는 단백질 분획을 모았고 활성도와 일치하는 분획을 얻었다. 전기영동으로 관찰한 결과 $Go{\alpha}$가 분자량 39,000 dalton. $G{\beta}$가 36,000 dalton인 band를 확인하였고 나머지 다른 단백질도 함께 관찰되어 heptylamine-Sepharose 분획을 다시 DEAE-Sephacel column에 적용하여 순수한 band를 구하였다. GTP 결합단백질의 활성화는 GTP가 결합될 때 ${\alpha}$부분과 결합하고 ${\beta}{\gamma}$는 떨어져 나간다. 그러므로 heptylamine-Sepharose column분획의 활성도에서 $Go{\alpha}$의 band 분획과 곡선의 활성도가 일치하고 ${\beta}$는 곡선이 하향하는 분획에서 전기영동상에 관찰되었다.

• 대한약리학회지
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• 제32권2호
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• pp.151-158
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• 1996

Following the subcutaneous administration of $R(-)N^6-(2-phenylisopropyl)adenosine(600\;nmol/kg/hr)$ to rats for 1 week using t$Alzet^{\circledR}$ mini-osmotic pumps, $A_1$ adenosine receptor functions were determined using $[^3H]DPCPX$ binding, $[^{35}S]GTP_{\gamma}S$ binding, and adenylyl cyclase assays. $A_1$ adenosine receptor binding and the inhibition of adenylyl cyclase activity by PIA was not altered in cerebrocortical membranes prepared from PIA-treated rats. However, there was a significant decrease in the $A_1$ adenosine receptor-mediated stimulation of $[^{35}S]GTP_{\gamma}S$ binding to cerebrocortical membranes prepared from PIA-treated rats(22.0% decrease in basal activity; 19.7% decrease in maximal activity). These results suggest that the desensitization of $A_1$ adenosine receptors following chronic administration involves agonist-induced uncoupling of the receptors from G proteins rather than alteration of $A_1$ adenosine receptor molecules. It is also suggested that the determination of stimulation of $[^{35}S]GTP_{\gamma}S$ binding to G proteins is a suitable tool in studying the receptor regulation including desensitization

• BMB Reports
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• 제34권2호
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• pp.95-101
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• 2001

Tissue transglutaminase (TGII, $G{\alpha}h$) belongs to a family of enzymes which catalyze post-translational modification of proteins by forming isopeptides via $Ca^{2+}$-dependent reaction. Although TGII-mediated formation of isopeptides has been implicated to play a role in a variety of cellular processes, the physiological function of TGII remains unclear. In addition to this Tease activity, TGII is a guanosine triphosphatase (GTPase) which binds and hydrolyzes GTP It is now well recognized that the GTPase action of TGII regulates a receptor-mediated transmembrane signaling, functioning as a signal transducer of the receptor. This TGII function signifies that TGII is a new class of GTP-binding regulatory protein (G-protein) that differs from "Classical" heterotrimeric G-proteins. Regulation of enzyme is an important biological process for maintaining cell integrity. This review summarizes the recent development in regulation of TGII that may help for the better understanding of this unique enzyme. Since activation and inactivation of GTPase of TGII are similar to the heterotrimeric G-proteins, the regulation of heterotrimeric G-protein in the transmembrane signaling is also discussed.

• 대한약리학회지
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• 제32권1호
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• pp.23-29
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• 1996

전통적인 수용체 이론에 따르면 상경적 길항제는 효현제와 수용체의 같은 부위에 작용하지만, 효능(efficacy)이 없기 때문에 생물학적 반응을 일으키지는 않는다. 그러나 최근에 발표되는 자료들에 따르면 모든 길항체의 효능(efficacy)이 0가 아니라 음수도 될 수가 있다고 생각된다. 이러한 음수의 효능을 갖는 약물을 역효현제라 부른다. 본 연구에서는 쥐의 cerebral cortex에서 얻은 membranes을 사용하여, $A_1$ 아데노신 수용체에 작용하는 역효현제를 인구하였다. 8개의 길항제로 알려진 약물들이 G단백에 대한 $[^{35}S]GTP_{\gamma}S$ 결합을 감소시키는 정도를 측정함으로써 역효현제의 특성을 검색하였다. 효현제에 의한 $[^{35}S]GTP_{\gamma}S$ 결합의 증가는 이틀 길항제틀에 의해 완전히 억제되었지만, 검색한 8개의 길항제는 두 군으로 구분되었다. DPCPX를 포함한 7개 길항제는 효현제 부재시의 basal $[^{35}S]GTP_{\gamma}S$ binding을 통계적으로 의의있게 감소시켜 역효현제의 특성을 나타내는 반면, CCS-15943은 basal $[^{35}S]GTP_{\gamma}S$ binding에 아무런 영향을 주지 않았다. NEM을 membranes에 처치하면 PIA에 의한 $[^{35}S]GTP_{\gamma}S$ binding이나 basal binding 둘다 감소하는데 이는 $[^{35}S]GTP_{\gamma}S$ binding의 상당부분이 G단백의 activated state를 나타내는 것을 알 수 있다. 또한 $[^3H]DPCPX$를 이용한 competitive binding assay에서 0.1 mM GTP는 효현제인 PIA의 apparent affinity를 감소시켰으며, DPCPX의 apparent affinity는 증가시키고, CGS-15943에는 아무런 영향을 미치지 않았다. 이것은 상기의 $[^{35}S]GTP_{\gamma}S$ binding의 결과를 뒤받침해 주는 결과라고 생각된다.

• Molecules and Cells
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• 제25권3호
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• pp.385-389
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• 2008

Septins are a family of filament-forming GTP-binding proteins involved in a variety of cellular process such as cytokinesis, exocytosis, and membrane dynamics. Here we report the biochemical and immunocytochemical characterization of a recently identified mammalian septin, SEPT12. SEPT12 binds GTP in vitro, and a mutation (Gly56 to Asn) in the GTP-binding motif abolished binding. Immunocytochemical analysis revealed that wild-type SEPT12 formed filamentous structures when transiently expressed in Hela cells whereas $SEPT12^{G56A}$ generated large aggregates. In addition, wild-type SEPT12 failed to form filaments when coexpressed with $SEPT12^{G56A}$. We also observed that GTP-binding by SEPT12 is required for interaction with SEPT11 but not with itself.