• Tuberculosis and Respiratory Diseases
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• 제45권4호
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• pp.846-860
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• 1998

연구배경: 내독소는 생체 내에서 단구와 내피세포에 강한 자극을 주나 호중구, 림프구, 호염기구, 섬유모세포 등 여러 세포에도 자극효과가 있어 염증반응이 시작된다. 그중 대식세포는 내독소의 자극을 받아 활성화되면 interleukin-1 (IL-1), IL-6, tumor necrosis factor-alpha (TNF-$\alpha$)를 분비하여 조직손상을 일으킨다. 내독소의 작용기전은 CD14 의존성 경로와 비의존성 경로의 두 개로 나뉘어진다. 체내로 들어온 내독소는 혈청 내에서 내독소 운반에 관여하는 LPS-binding protein(LBP)과 결합하여 혈중내에서 세포와 결합되거나 조직으로 이동되어 조직내 세포와 결합하게 된다. 그러나 고농도의 LPS는 CD14항원에 비의존적으로 대식세포를 자극 할 수 있는 것으로 알려져 있다. 현재까지 LPS자극에 의한 대식세포의 CD14 항원 의존성 IL-1, IL-6, TNF-$\alpha$의 형성과정은 많이 밝혀져 있으나, 내독소에 의한 TGF-$\beta$의 형성 여부는 밝혀져 있지 않으며, CD14 항원 비의존성으로 IL-1, IL-6, TNF-$\alpha$ TGF-$\beta$가 형성되는 과정도 별로 밝혀져 있지 않다. 본 연구에서는 혈청이 없는 상태 (LBP가 없는 상태)에서, 즉 LPS 자극시 LBP-CD14 비의존성으로 말초혈액단핵구에서 형성된 proinflammatory cytokines인 IL-1, IL-6, TNF-$\alpha$과 섬유화 cytokine인 TGF-$\beta$의 생성유무를 규명하고자 하였다. 방 법: 정상인의 헤파린 처리된 말초혈액정맥혈을 비중 1.077의 Ficoll-Hypaque 용액 위에 중첩시킨 후 500g에서 30분간 원심분리하여 말초혈액단핵구를 얻었다. 분리된 말초혈액단핵구를 우태아혈청이 없는 RPMI에 부유시킨 후 $37^{\circ}C$, 5% $CO_2$ 보온기에서 0.1 ${\mu}g$, 1 ${\mu}g$, 10 ${\mu}g$, 100 ${\mu}g/ML$의 LPS와 1, 2, 4, 8, 12, 24, 48 시간 혼합 배양 후 상층액을 분리하여 IL-6, TNF-$\alpha$, TGF-$\beta$의 측정 cytokines의 양을 bioassay로 측정하였다. 세포층은 slide에 고정시킨 후 단 클론 항체를 이용한 이중 면역조직화학염색법과 RNA probe를 이용한 in situ hybridization에 이용하였다. 결 과: 실험사약내 내독소 존재 여부에 대한 검증결과 내독소 함유량은 10 ng/mL 이하로 되어 있어 본 실험에서는 10 ng/mL 이상의 농도로 실험을 하였기 때문에 오염된 내독소는 실험에 영향이 없었을 것으로 사료되었다. 말초혈액단핵구에서 LPS 자극에 의하여 IL-6는 1시간째부터 형성되기 시작하였으며 96 시간까지 지속적으로 상승하였고 LPS용량의존성으로 형성됨을 알 수 있었다. TNF-$\alpha$는 LPS 자극 4시간째부터 상승하기 시작하여 시간이 갈수록 생성양은 증가하며 72 시간째까지 지속적으로 형성되었다. TGF-$\beta$형성도 LPS 용량에 의존성을 보이며 8시간째 일차로 TGF-$\beta$의 형성이 증가 한 후 12 시간째는 오히려 감소하였다가 시간이 지남에 따라 다시 증가하여 2차로 96 시간에 최대 형성을 보였다. 각각 cytokine의 24시간째 생성양은 IL-6의 경우 $1{\times}10^5/mL$의 말초혈액단핵구에서 10 ${\mu}g/mL$의 LPS에 의해서 19.8 ng 이 생성되었고 LPS 자극이 없는 상태의 자연생성능도 3.2 ng이었으며, $1{\times}10^6/mL$의 말초혈액단핵구에 의해서 자연 생성양은 증가하여 24시간째에 0.38 ng/mL, 10명/mL의 농도에서 24시간째 4.1 ng/mL의 TNF-$\alpha$의 생성능을 보였다. TGF-$\beta$의 경우 $2{\times}10^6/mL$의 말초혈액단핵구에 의하여 34.4 pg/mL가 생성되었고 자연생성능은 5.2 pg/mL의 생성농을 보였다. 말초혈액단핵구의 IL-1$\beta$, IL-6, TNF-$\alpha$, TGF-$\beta$ 단백과 m-RNA 발현 IL-1$\beta$, IL-6, TNF-$\alpha$단백은 주로 단구세포에서, TGF-$\beta$ 단백은 단구세포와 림프구에서 발현되었으며, CD14항원 발현과는 상관이 없었다. TNF-$\alpha$, IL-1$\beta$, IL-6, TGF-$\beta$ m-RNA 양성세포는 주로 세포질이 풍부한 것으로 보아 단구세포로 사료되었다. TGF-$\beta$의 경우 단구세포외에도 세포질이 적은 림프구에서도 약하게 양성반응을 보여 링프구에서도 분비될 가능성을 보여 주었다. 결 론: 내독소로 말초혈액 단핵구를 자극시 IL-6, TNF-$\alpha$는 조기에 분비되기 시작하며 TGF-$\beta$는 후기에 분비되기 시작하여 96시간까지 지속적으로 분비된다. 주 분비세포는 IL-1$\beta$, IL-6, TNF-$\alpha$의 경우 단구세포가 되며 TGF-$\beta$도 단구세포가 주세포가 되나 림프구도 분비에 관여한다.

• 한국미생물·생명공학회지
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• 제25권2호
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• pp.137-143
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• 1997

Porcine transforming growth factor-$\beta$1 (TGF-$\beta$1) was expressed in Escherichia coli using cDNA of TGF-$\beta$1 and glutathione S-transferase (GST) fusion vector pGEX-1$\lambda$T. An ApoI-Tth111I fragment of cDNA which correspond to the amino acid residues from 123 to 390 of the precursor TGF-$\beta$1 was inserted into EcoRI-Tth111I digested pGEM#-l$\lambda$T and the recombined plasmid was named pGET-12. Gene products from the cloned regions of the recombinant plasmids pGET-12 was not detected in soluble fraction of cell free extract but detected in insoluble fraction. The solubilization of insoluble gene product was achieved by the treatment of N-laurylsarcosine. Molecular weight of partially purified proteins determined by electrophoresis was same as expected from cloned fragment. The ELISA test results of the purified proteins showed that immunologically detectable epitope was preserved in recombinant protein.

• Journal of the Korean Association of Oral and Maxillofacial Surgeons
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• 제26권4호
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• pp.345-354
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• 2000

TGF-${\beta}_1$ is a potent chemotactic factor for inflammatory cells and fibroblasts. It also stimulates the celluar source and components of extracellular matrix and the production of proteinase inhibitors. Collectively, these biologic activities lead to the accumulation and stabilization of the nascent matrix, which is vital to wound healing. The objective of this study is to investigate production of TGF-${\beta}_1$ in vitro fibroblast culture in the presence of Staphylococcus enterotoxin B(SEB) and/or lipopolysaccharide(LPS) and to elucidate the role of TGF-${\beta}_1$ which may be responsible for wound healing. The fibroblasts were originated from facial dermis and hypertrophic scar in 26 year-old male patient. In the presence of LPS($0.01{\mu}g$, $0.1{\mu}g$, $1.0{\mu}g$), SEB($0.01{\mu}g$, $0.1{\mu}g$, $1.0{\mu}g$) respectively, cells($5{\times}10^3ml$) were cultivated in vitro. At 1, 3, and 5 days after incubation, cells were counted. Also, cells($2.5{\times}10^5ml$) were cultivated in EMEM with LPS(0.01, 0.1 and $1.0{\mu}g$), SEB(0.01, 0.1 and $1.0{\mu}g$) respectively and LPS($0.1{\mu}g$) and SEB($0.1{\mu}g$) in combination for 24, 48, and 72 hours respectively. Culture supernatants were harvested at 1, 2, and 3 days after incubation period and triplicate culture supernatants were pooled and TGF-${\beta}_1$ was assayed in duplicate. The results were as follows. 1. In facial dermal fibroblast induced with SEB and LPS respectively or in combination, the suppression of cell proliferation occurred very significantly at 1 day after incubation, compared with the control. In SEB exposure, the production of TGF-${\beta}_1$ was decreased very significantly at 1 day after incubation, compared with the control. However, in LPS, SEB and LPS exposure, the production of TGF-${\beta}_1$ was increased very significantly at 1 day after incubation, compared with the control. 2. In hypertrophic scar fibroblast induced with SEB and LPS respectively or in combination, the suppression of cell proliferation did not occur at 1 day after incubation, compared with the control. In SEB and LPS exposure in combination, the production of TGF-${\beta}_1$ was increased very significantly at 1 day after incubation, compared with the control. However, the production of TGF-${\beta}_1$ did not occur in SEB and LPS exposure respectively. In conclusion, the concentration of bacterial toxins and the incubation period correlated with cell proliferation and production of TGF-${\beta}_1$ very significantly and both fibroblasts have different phenotype each other in this regard. This data suggest that the significant production of TGF-${\beta}_1$ may develope abnormal wound healing associated with tissue fibroproliferative disorder, such as hypertrophic scar and keloid formation.

• BMB Reports
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• 제50권8호
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• pp.429-434
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• 2017

Endometriosis is the abnormal growth of endometrial cells outside the uterus, causing pelvic pain and infertility. Furthermore, adhesion of endometrial tissue fragments to pelvic mesothelium is required for the initial step of endometriosis formation outside uterus. $TGF-{\beta}1$ and adhesion molecules importantly function for adhesion of endometrial tissue fragments to mesothelium outside uterus. However, the function of $TGF-{\beta}1$ on the regulation of adhesion molecule expression for adhesion of endometrial tissue fragments to mesothelium has not been fully elucidated. Interestingly, transforming growth factor ${\beta}1$ ($TGF-{\beta}1$) expression was higher in endometriotic epithelial cells than in normal endometrial cells. The adhesion efficiency of endometriotic epithelial cells to mesothelial cells was also higher than that of normal endometrial cells. Moreover, $TGF-{\beta}1$ directly induced the adhesion of endometrial cells to mesothelial cells through the regulation of integrin of ${\alpha}V$, ${\alpha}6$, ${\beta}1$, and ${\beta}4$ via the activation of the $TGF-{\beta}1/TGF-{\beta}RI/Smad2$ signaling pathway. Conversely, the adhesion of $TGF-{\beta}1-stimulated$ endometrial cells to mesothelial cells was clearly reduced following treatment with neutralizing antibodies against specific $TGF-{\beta}1-mediated$ integrins ${\alpha}V$, ${\beta}1$, and ${\beta}4$ on the endometrial cell membrane. Taken together, these results suggest that $TGF-{\beta}1$ may act to promote the initiation of endometriosis by enhancing integrin-mediated cell-cell adhesion.

• 대한본초학회지
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• 제28권4호
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• pp.49-55
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• 2013

Objectives : Mori Folium was popularly used as one of the traditional medicinal herbs. Although M. Folium has been cultivated for rearing silkworm historically, it's use has been expanded as natural therapeutic agent for the treatment of filariasis, diabetes and dropsy in East Asia. However, little has been known about the effect of M. Folium on liver fibrosis. Therefore, we would like to explore an anti-fibrogenic potential of M. Folium extract (MFE) using immortalized human hepatic stellate cell line, LX-2 cells. Methods : We examined the effects of MFE on the transforming growth factor ${\beta}1$ ($TGF{\beta}1$)-induced liver fibrosis in LX-2 cells. Cell viability, Smad binding element-driven luciferase activity, phosphorylations level of Smad 2/3, and expression level of $TGF{\beta}1$-dependent target genes were monitored in the MFE-treated LX-2 cells. Results : Up to 30 ${\mu}g/ml$ MFE treatment did not show any possible toxic effect in LX-2 cells. MFE inhibited $TGF{\beta}1$-inducible Smad binding element-driven luciferase activity and decreased the $TGF{\beta}1$-inducible phosphorylations of Smad 2 and Smad 3 in hepatic stellate cell in a dose dependent manner. Furthermore, increases of plasminogen activator inhibitor type 1, $TGF{\beta}1$ and matrix metalloproteinases 2 genes by $TGF{\beta}1$ were also attenuated by MFE treatment. Conclusions : These findings suggested that MFE would be used as a potential therapeutic agent for the treatment liver fibrosis, which might be mediated by the inhibition of $TGF{\beta}1$-inducible Smad 2/3 transactivation and target genes expression.

• Experimental and Molecular Medicine
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• 제50권12호
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• pp.4.1-4.19
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• 2018

Transforming growth factor $(TGF)-{\beta}$ signaling is increasingly recognized as a key driver in cancer. In progressive cancer tissues, $TGF-{\beta}$ promotes tumor formation, and its increased expression often correlates with cancer malignancy. In this study, we utilized adenoviruses expressing short hairpin RNAs against $TGF-{\beta}1$ and $TGF-{\beta}2$ to investigate the role of $TGF-{\beta}$ downregulation in cancer cell death. We found that the downregulation of $TGF-{\beta}$ increased the phosphorylation of several SAPKs, such as p38 and JNK. Moreover, reactive oxygen species (ROS) production was also increased by $TGF-{\beta}$ downregulation, which triggered Akt inactivation and NOX4 increase-derived ROS in a cancer cell-type-specific manner. We also revealed the possibility of substantial gene fluctuation in response to $TGF-{\beta}$ downregulation related to SAPKs. The expression levels of Trx and GSTM1, which encode inhibitory proteins that bind to ASK1, were reduced, likely a result of the altered translocation of Smad complex proteins rather than from ROS production. Instead, both ROS and ROS-mediated ER stress were responsible for the decrease in interactions between ASK1 and Trx or GSTM1. Through these pathways, ASK1 was activated and induced cytotoxic tumor cell death via p38/JNK activation and (or) induction of ER stress.

• 대한약학회:학술대회논문집
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• 대한약학회 2003년도 Proceedings of the Convention of the Pharmaceutical Society of Korea Vol.2-2
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• pp.152.2-153
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• 2003

${\beta}Although$ it has been demonstrated that $p2l^{WAFl/Cip1}$, a well known cell cycle inhibitor, could be induced by $TGF-{\beta}$ in a p53-independent manner, the detailed signal transduction pathways still remain poorly understood. In this study, we show that ERK is required for $TGF-{\beta}$ induction of $p21^{WAF1/Cip1}$, but JNK or p38 MAPK is not. ERK activation by $TGF-{\beta}$ significantly attenuated by treatment with ROS scavenger such as NAC or catalase, indicating that ROS, mainly $H_2O_2$, generation by $TGF-{\beta}$ might stimulate ERK signaling pathway to require the induction of $p21^{WAF1/Cip1}$. (omitted)

• Asian Pacific Journal of Cancer Prevention
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• 제17권5호
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• pp.2429-2434
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• 2016

Transforming growth factor-B1 ($TGF-{\beta}1$ )and its coreceptor endoglin (ENG) have been shown to contribute to hepatocellular tumor development and malignant progression. Our aim was to evaluate the serum expression levels of $ENG/TGF-{\beta}1$ mRNAs and risk of hepatocellular carcinoma in cirrhotic Egyptian patients. Our study included 77 subjects. Real time polymerase chain reaction was used to evaluate the expression level of ENG and $TGF-{\beta}1$mRNAs. The relative expression ratio of ENG mRNA was 0.82 (0.1 -3.2), 0.66 (0.15-5.3), 0.38(0.007-2.8) and 0.12 (0.00-0.22) and the relative expression ratio of $TGF-{\beta}1$mRNA was 1.4 (0.19 -6.2), 1.2 (0.22-4.3), 1.0 (0.15-4.4) and 0.6 (0.00-2.2) for cirrhotic HCC cirrhotic, HCC only and healthy control groups respectively. Increased ENG and $TGF-{\beta}1$ mRNA gene expression was correlated with TNM clinical stage. The expression ratio in TNM stage III-IV 1.1 (0.07-3.2), 1.55 (0.15-6.2) was statistically significantly higher than that in stage I-II 0.47 (0.007-2.8), 1.0 (0.31-4.4) (P<0.05). Our data suggested that increased ENG and $TGF-{\beta}1$ gene expression may participate in hepatocarcinogenesis and increased risk of HCC in individuals with cirrhosis. Early screening for evidence of cirrhosis and consideration of ENG and $TGF-{\beta}1$ as targets for therapy and treatment strategies are warranted.

• Journal of Microbiology and Biotechnology
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• 제12권1호
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• pp.65-70
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• 2002

A TGF-${\beta}1$/GFP monomeric fusion protein was cloned from pPK9A and pGFP-Cl plasmid by PCR amplification. The fusion protein was expressed in a $Bac-To-Bac^{TM}$ baculovirus expression system. A 45 kDa fusion protein was purified using an Ni-NTA column with 300 mM imidazol from a cell lysate infected with recombinant viruses for 72 h post-infection. The fusion protein cross-reacted with the commercial $TGF-{\beta}1$ polyclonal Ab as well as Ab raised against a precursor, monomeric $TGF-{\beta}1$, and GFP. The binding activity of the fusion protein with a $TGF-{\beta}1$ receptor was examined. Fluorescence was observed in Mv1Lu cells, yet not in insect cells treated with the fusion protein. No fluorescence was detected in Mv1Lu cells incubated with the fusion protein treated with Ab prior to the binding reaction, or with GFP alone, thereby indicating that the binding of the fusion protein was specific to $TGF-{\beta}1$ with a receptor.

• 한국가축번식학회지
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• 제20권2호
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• pp.111-117
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• 1996

본 연구는 혈청첨가 또는 무첨가에 따른 소 난포란의 체외성숙에 있어서 참가된 TGF-$\beta$1과 IGF-I이 그후의 수정 및 발생에 미치는 영향과, 이들 growth factor의 농도에 따른 8세포기 소 체외수정란의 발달에 미치는 영향을 조사하고자 실시하였다. 도축장에서 얻어진 난소로부터 채취된 난포란을 20% FBS가 첨가 또는 첨가되지 않은 TCM-199에 TGF-$\beta$1, IGF-I 또는 TGF-$\beta$1＋IGF-I을 각각 10ng/ml 첨가하여 38.5$^{\circ}C$에서 24시간 배양하여 체외성숙을 유기하였다. 성숙된 난자를 1$\times$106/ml 정자농도로 수정후 24시간에 glucoserk 첨가되지 않은 CZB 배양액으로 옮겨 48시간 배양한 다음, TCM-199＋20%FBS에서 96시간 추가배양하였다. 본 연구에서 혈청이 첨가된 난포란의 체외성숙배양액에 첨가된 growth factor들은 수정후의 배분할 및 배발생에 영향을 미치지 않았다. 혈청이 첨가되지 않은 경우에서는 TGF-$\beta$1의 첨가는 배분할 및 배발생율을 향상시켰다(P<0.05). 한편 TCM-199＋20%FBS에 5, 10ng/ml의 TGF-$\beta$1 및 5, 10, 50, 100ng/ml의 IGF-I을 각각 첨가후 8세포기 체외수정란을 배양한 결과, 10ng/ml TGF-$\beta$1의 첨가는 배반포기로의 발생율을 향상시켰다(P<0.05). 결론적으로, 혈청이 포함되지 않은 소 난포란의 체외성숙 배양액, 또는 수정란의 체외배양액에 10ng/ml TGF-1의 첨가는 배반포기로의 발생율을 향상시킨다.