• Parasites, Hosts and Diseases
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• 제33권3호
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• pp.155-164
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• 1995

Cyptosporidium parvum의 발달 단계별 actin과 myosin의 분포 위치를 면역황금염색법을 이용하여 관찰하였다. $Depomedrol^{\circledR}$을 ICR마우스에 피하주사하여 면역억제시킨 후 C. parvum이 발현된 마우스 회장을 잘라 LR gold로 포매하여 초박절편을 떴다. 일차항체로는 chickenbackmuscle actin과 bovine uterus myosin에 대한 rabbit polyclonal antibody를 사용하였고 이차항체로는 10 mm 크기의 황금입자가 결합된 goatanti-rabbit lgG를 반응시켰다 Uranylacetate와 leadcitrate로 염색한 후 투과전자현미경으로 관찰하였다 Trophozoite에서는 세포막에서 주로 actin과 myosin이 관찰되었고 feederorganelle 주위 세포질에는 actin이 분포하였다. Meront와 같이 활발히 분열하고 있는 단계에서는 세포막과 세포질 전체에 actin이 분포되어있었으며 myosin은 세포막에서만 소량 관찰되었다. 핵과 anlage of rhoptries 등은 두 단백질에 모두 염색되지 않았다. Macrogametocyte 에서는 amylopectin-lile bodies에서 actin과 myosin이 모두 관찰되었으나 wall forming bodies에서는 관찰되지 않았고 feederorganelle 주위 세포질 부분에서는 actin이 관찰되었다. Sporozoite를 포함하는 oocyst와 merozoite를 포함하는 meront에서는 세포막과 세포막사이에서 actin이 다수 관찰 되었으며 myosin은 소량 관찰되었다. Merozoites가 빠져나가 속이 비어있는 parasitophorous vacuole중에는 microspike를 형성한 것들이 종종 관찰되었고 이것이 좀더 길어져 마치 microvilli와 같이 보이는 경우도 있었으며 이러한 구조물에서도 actin이 다수 관찰되었다. 이상의 결과로 미루어 actin과 myosin은 세포막에 주로 분포하면서 C. parvum의 형태를 유지시키며 또한 세포막의 움직임을 조절하는 cytoskeletalproteiA으로서의 역할이 주된 작용일 것으로 생각되었다.

• 한국정보기술학회 영문논문지
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• 제9권1호
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• pp.103-113
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• 2019

Motivation: Polymerized actin-based cytoskeletal structures are crucial in shape, dynamics, and resilience of a cell. For example, dynamical actin-containing ruffles are located at leading edges of cells and have a significant impact on cell motility. Other filamentous actin (F-actin) bundles, called stress fibers, are essential in cell attachment and detachment. For this reason, their mechanistic understanding provides crucial information to solve practical problems related to cell interactions with materials in tissue engineering. Detecting and counting actin-based structures in a cellular ensemble is a fundamental first step. In this research, we suggest a new method to characterize F-actin wrapping fibers from confocal fluorescence image stacks. As fluorescently labeled F-actin often envelope the fibers, we first propose to segment these fibers by diminishing an energy based on maximum flow and minimum cut algorithm. The actual actin is detected through the use of bilateral filtering followed by a thresholding step. Later, concave actin bundles are detected through a graph-based procedure that actually determines if the considered actin filament is enclosing the fiber.

• International Journal of Oral Biology
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• 제30권1호
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• pp.17-22
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• 2005

In the previous studies of Saccharomyces cerevisiae, Abp140p (actin binding protein 140) fused to GFP has been only a protein that can label actin cables of yeast cells so far. However, the role of Abp140p in actin dynamics was remained elusive. In this study, the function of Abp140p was investigated with a deletion mutant and overexpression of GFP fused Abp140p. The deletion mutant was slightly more susceptible to Latrunculin-A (Lat-A), an actin-monomer sequestering agent, than wild type, although no significant deformation of actin structures was caused by ABP 140 deletion. Overexpression of Abp140p-GFP retarded cell growth, and produced thick and robust actin cables. Lat-A was not able to destabilize the thick actin cables, which suggests that actin dynamics was compromised in the cells with surplus of Abp140p. Therefore, Abp140p seems to stabilize actin cables together with other bundling proteins. Recently, actin cable dynamics of budding yeast was found to have a resemblance to that of filopodial tip of cultured mammalian cells. Retrograde movement of actin cables from buds to mother cells indicated local generation of the cable at bud sites. By using Abp140p-GFP, we traced the steps in the generation of a new actin cable after elimination of old cables by sodium azide. Before the appearance of a new actin cable, Abp140p-GFP concentrated in buds and disappeared, as mother cells became abundant in actin cables. Our observations provide a direct evidence of actin cable formation at buds of budding cells.

• Journal of Microbiology
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• 제39권1호
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• pp.42-48
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• 2001

The regulation of actin gene expression during the differentiation of Naegleria gruberi was examined. Actin mRNA concentration was maximal in amoebae and decreased rapidly after the initiation of differentiation. At 20 min after initiation, the concentration of actin mRNA decreased to 55% of the maximal value. The actin mRNA concentration decreased to the minimum at 80 min (15% of the maximum), and then began to increase slightly at the end of differentiation. This decrease of actin mRNA concentration was regulated by the repression of actin gene transcription based on nuclear run-on transcription experiments. The rates of transcription of actin gene in nuclei prepared at 40 and 80 min after the initiation of differentiation were 50 and 28% of that of nuclei prepared at the beginning of differentiation, respectively. The addition of cycloheximide at the initiation of differentiation inhibited both the rapid decrease in the concentration of actin mRNA and the repression of actin gene transcription. These results suggest that the rapid decrease in the concentration of actin mRNA during the differentiation of N. gruberi is accomplished by the repression of actin gene transcription and this transcriptional regulation requires continuous protein synthesis during the differentiation.

• 한국어류학회지
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• 제17권1호
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• pp.49-56
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• 2005

점박이송사리, Rivulus marmoratus에서 기원된 16개의 ${\beta}-actin$ 유전자의 염기서열 분석 결과 1,764~1,769 bp 범위를 가지는 ${\beta}-actin$ 유전자를 분리하였다. 이는 기존에 보고된 점박이송사리 ${\beta}-actin$ 유전자와 exon 1 및 intron 2지역에서 다소의 차이를 보여 우리는 이를 점박이송사리 ${\beta}-actin$ 2 유전자라 명명하였다. Multiple alignment를 이용하여 유전자 서로간의 차이를 비교한 결과, 점박이송사리 ${\beta}-actin$ 유전자는 variation을 볼 수 있었다. 따라서 본 연구에서는 점박이송사리에 있어 ${\beta}-actin$ 유전자의 종내 변이 (intraspecific variation)를 확인하였다.

• 생명과학회지
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• 제8권6호
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• pp.681-686
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• 1998

이상의 결과로부터 spin lavel의 영향은 IASL, MSL은 이완상태 myosin head의 규칙적인 나선 배열은 흐트러진다. 특히 IASL은 효과가 크다. 적도반사의 변화로부터 myosin head는 spin label하는 것에 의해 actin filament 근방에 이동해 있다는 것을 알 수 있었다. 215 $\AA$ 반사의 감소는 spin lavel에 의한 myosin의 143 $\AA$주기성을 더욱 강하게 해 준다. 143 $\AA$, 72 $\AA$의 거동은 filament축으로부터 투영한 구조를 반영하기 때문에 IASL에는 143 $\AA$ 주기의 밀도분포가 완만하게 되어 있다는 것을 나타내고, MSL에는 143 $\AA$ 분포가 올라와 있다는 것을 나타낸다. actin 반사변화에서 MSL의 actin반사의 증가는 이동한 myosin head가 어떤 actin과 결합하였거나, spin lavel의 영향으로 actin의 구조가 변화되었다. 한편, IASL은 actin반사를 감소 시키기 때문에 myosin head의 결합을 하지 않았다. 결론적으로, 이것은 actin의 SH기에도 spin label되어 actin의 나선 구조가 크게 흐트러짐을 알 수 있었다

• 한국자원식물학회지
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• 제28권5호
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• pp.648-655
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• 2015

본 연구에서는 도라지의 품종 구분 및 유전적 다양성 분석에 활용될 수 있는 분자표지 개발을 위하여 RAPD 마커를 활용하여 분석하였으며, 동시에 actin유전자 염기서열에서 유래한 분자표지를 제작하였다. 총 30개의 RAPD 분자표지를 활용한 분석을 진행하였으나, 재현성과 안정성이 확보된 DNA 상의 다형성은 확보할 수 없었다. 이에, 도라지 actin (Pg-actin) 유전자에 존재하는 Single Nucleotide Polymorphism (SNP)을 이용하여 품종 간 구분에 활용 가능한 분자마커로의 전환을 탐색하였다. 도라지 genomic DNA에 actin 유래 유전자를 사용하여 2개의 actin homologs를 확보하였으며, 이를 염기서열 분석하여 3.4 kb의 Pg-actin fragment와 Pg-actin과 28.6%의 유사도를 가진 1.4 kb의 actin homologue를 획득하였다. 획득된 Pg-actin은 4개의 exon과 3개의 intron으로 구성된 유전자로, DNA 다형성 탐색을 통해 intron 3의 286 bp 위치에서 SNP (G ↔ A)를 발견하였으며, 이를 활용도 높은 CAPS marker로 전환하여 PgActin-Int3 마커를 개발하였다. Pg-Actin-Int3 마커를 32개의 도라지 유전자원에 적용시켜 본 결과 품종 간의 차이를 보이는 부분이 확인되었다. 본 연구에서 확보된 도라지 DNA 염기서열정보는 도라지의 유전적 다양성 분석 및 도라지 분자육종에 활용될 수 있을 것이라 전망된다.

• BMB Reports
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• 제48권7호
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• pp.369-370
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• 2015

Actin dynamics is critical for the formation and sustainment of the immunological synapse (IS) during T cell interaction with antigen-presenting cells (APC). Thus, many actin regulating proteins are involved in spatial and temporal actin remodeling at the IS. However, little is known whether or how actin stabilizing protein controls IS and the consequent T cell functions. TAGLN2 − an actin-binding protein predominantly expressed in T cells − displays a novel function to stabilize cortical F-actin, thereby augmenting F-actin contents at the IS, and acquiring leukocyte function-associated antigen-1 activation following T cell activation. TAGLN2 also competes with cofilin to protect F-actin in vitro and in vivo. During cytotoxic T cell interaction with cancer cells, the expression level of TAGLN2 at the IS correlates with the T cell adhesion to target cancer cells and production of lytic granules such as granzyme B and perforin, thus expressing cytotoxic T cell function. These findings identify a novel function for TAGLN2 as an actin stabilizing protein that is essential for stable immunological synapse formation, thereby regulating T cell immunity. [BMB Reports 2015; 48(7): 369-370]

• 한국양식학회지
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• 제22권1호
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• pp.83-91
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• 2009

The Korean doty barbel Hemibarbus mylodon (Cypriniformes; Cyprinidae) is a critically endangered freshwater fish species mainly because of its natural habitat degradation. Three full-length complementary DNA (cDNA) clones representing different muscle actin isoforms were isolated and characterized. The three muscle actin isoforms were 1,294-1,601 bp long with the identical open reading frames of 1,134 bp with the deduced amino acid residues of 377. They showed 83.9-87.2% identities in the coding nucleotide level and 96.8-98.1% identities in the amino acid level. Phylogenetic analysis with the coding nucleotide sequences revealed that three muscle actin isoforms of H. mylodon formed strongly supported monophyletic groups with one of cypriniform skeletal $\alpha$-actin (acta1), cypriniform aortic $\alpha$-actins (acta2), and uncharacterized Danio rerio muscle actin isoform/Salmo trutta slow muscle actin (a novel muscle actin type). Our phylogenetic tree further suggested that cypriniform acta2 only showed the orthologous relationship to tetrapod acta2. Other multiple actin isoforms from diverse teleostean taxa were however clustered to no tetrapod orthologs, i.e., acta1, cardiac $\alpha$-actins (aetc1), acta2, and enteric $\gamma$-actin (actg2). This result strongly suggested that teleostean muscle actins have experienced different and complicated evolutionary history in comparison to mammalian counterparts.

• BMB Reports
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• 제29권4호
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• pp.353-358
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• 1996

Bovine angiogenin (bAng) is a potent blood vessel inducing protein purified from cow In ilk. fluorescence spectroscopy has been used to study the interaction of bAng with actin in 50 mM Tris-HCl pH 7.5, and 1 mM $CaCl_2$ at $25^{\circ}C$. Actin contains four tryptophans but bAng contains no tryptophans. A 50% decrease in intrinsic fluorescence accompanied formation of the bAng/actin complex. By contrast, the interaction of RNase A, a homologous protein to bAng, with actin results in about 10% quenching of the fluorescence. Fluorescence titration experiments were performed by adding increasing concentrations of bAng (0~1.0 ${\mu}M$) to a constant concentration of actin (0.1 ${\mu}M$), and the dissociation constant $K_d$ for the bAng/actin complex and the stoichiometry n were measured as $20{\pm}1$ nM and $1.0{\pm}0.1$ respectively. These results suggest that the interaction between bAng with actin is specific and that quenching of actin fluorescence has occurred in the bAng/actin complex. The bAng binding sites of actin are discussed in the results of this study, and we propose that Trp-80 in the small domain of bovine actin is responsible for the bAng/actin binding.