1.Wnt Signal Transduction and Its Involvement in Human Diseases.
Journal of Korean Society of Endocrinology 2005;20(4):306-318
No Abstract available.
Humans*
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Signal Transduction*
2.Pja2 Inhibits Wnt/β-catenin Signaling by Reducing the Level of TCF/LEF1
Yonghee SONG ; Somyung LEE ; Jeong Rae KIM ; Eek hoon JHO
International Journal of Stem Cells 2018;11(2):242-247
Ubiquitination of proteins plays an essential role in various cellular processes, including protein degradation, DNA repair, and cell signaling pathways. Previous studies have shown that protein ubiquitination is implicated in regulating pluripotency as well as fate determination of stem cells. To identify how protein ubiquitination affects differentiation of embryonic stem cells, we analyzed microarray data, which are available in the public domain, of E3 ligases and deubiquitinases whose levels changed during stem cell differentiation. Expression of pja2, a member of the RING-type E3 ligase family, was up-regulated during differentiation of stem cells. Wnt/β-catenin signaling is one of the most important signaling pathways for regulation of the self-renewal and differentiation of embryonic stem cells. Pja2 was shown to bind to TCF/LEF1, which are transcriptional factors for Wnt/β-catenin signaling, and regulate protein levels by ubiquitination, leading to down-regulation of Wnt signaling activity. Based on these results, we suggest that E3 ligase Pja2 regulates stem cell differentiation by controlling the level of TCF/LEF1 by ubiquitination.
DNA Repair
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Down-Regulation
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Embryonic Stem Cells
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Humans
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Ligases
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Proteolysis
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Public Sector
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Stem Cells
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Ubiquitin
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Ubiquitin-Protein Ligases
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Ubiquitin-Specific Proteases
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Ubiquitination
3.Negative feedback regulation of Wnt signaling by Gbetagamma-mediated reduction of Dishevelled.
Hwajin JUNG ; Hyun Joon KIM ; Suk Kyung LEE ; Rokki KIM ; Will KOPACHIK ; Jin Kwan HAN ; Eek hoon JHO
Experimental & Molecular Medicine 2009;41(10):695-706
Wnt signaling is known to be important for diverse embryonic and post-natal cellular events and be regulated by the proteins Dishevelled and Axin. Although Dishevelled is activated by Wnt and involved in signal transduction, it is not clear how Dishevelled-mediated signaling is turned off. We report that guanine nucleotide binding protein beta 2 (Gnb2; Gbeta2) bound to Axin and Gbeta2 inhibited Wnt mediated reporter activity. The inhibition involved reduction of the level of Dishevelled, and the Gbeta2gamma2 mediated reduction of Dishevelled was countered by increased expression of Axin. Consistent with these effects in HEK293T cells, injection of Gbeta2gamma2 into Xenopus embryos inhibited the formation of secondary axes induced either by XWnt8 or Dishevelled, but not by beta-catenin. The DEP domain of Dishevelled is necessary for both interaction with Gbeta2gamma2 and subsequent degradation of Dishevelled via the lysosomal pathway. Signaling induced by Gbeta2gamma2 is required because a mutant of Gbeta2, Gbeta2 (W332A) with lower signaling activity, had reduced ability to downregulate the level of Dishevelled. Activation of Wnt signaling by either of two methods, increased Frizzled signaling or transient transfection of Wnt, also led to increased degradation of Dishevelled and the induced Dishevelled loss is dependent on Gbeta1 and Gbeta2. Other studies with agents that interfere with PLC action and calcium signaling suggested that loss of Dishevelled is mediated through the following pathway: Wnt/Frizzled-->Gbetagamma-->PLC-->Ca+2/PKC signaling. Together the evidence suggests a novel negative feedback mechanism in which Gbeta2gamma2 inhibits Wnt signaling by degradation of Dishevelled.
Adaptor Proteins, Signal Transducing/genetics/*metabolism
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Animals
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Blastomeres/cytology/*metabolism
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Cell Line
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Embryonic Development/genetics
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*Feedback, Physiological
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Frizzled Receptors/genetics/metabolism
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GTP-Binding Proteins/genetics/*metabolism
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Gene Expression Regulation, Developmental
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Humans
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Mutation
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Phosphoproteins/genetics/*metabolism
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Protein Binding
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RNA, Small Interfering/genetics
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Repressor Proteins/genetics/metabolism
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Transfection
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Wnt Proteins/*genetics/metabolism
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Xenopus
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Xenopus Proteins/*genetics/metabolism
4.The Distinct Role of Tcfs and Lef1 in the Self-Renewal or Differentiation of Mouse Embryonic Stem Cells
Sewoon KIM ; Hanjun KIM ; Anderson TAN ; Yonghee SONG ; Hyeju LEE ; Qi-Long YING ; Eek-hoon JHO
International Journal of Stem Cells 2020;13(2):192-201
Background and Objectives:
Tcfs and Lef1 are DNA-binding transcriptional factors in the canonical Wnt signaling pathway. In the absence of β-catenin, Tcfs and Lef1 generally act as transcriptional repressors with co-repressor proteins such as Groucho, CtBP, and HIC-5. However, Tcfs and Lef1 turn into transcriptional activators during the interaction with β-catenin. Therefore, the activity of Tcfs and Lef1 is regulated by β-catenin. However, the intrinsic role of Tcfs and Lef1 has yet to be examined. The purpose of this study was to determine whether Tcfs and Lef1 play differential roles in the regulation of self-renewal and differentiation of mouse ES cells.
Methods:
and Results: Interestingly, the expression of Tcfs and Lef1 was dynamically altered under various differentiation conditions, such as removal of LIF, EB formation and neuronal differentiation in N2B27 media, suggesting that the function of each Tcf and Lef1 may vary in ES cells. Ectopic expression of Tcf1 or the dominant negative form of Lef1 (Lef1-DN) contributes to ES cells to self-renew in the absence of leukemia inhibitory factor (LIF), whereas ectopic expression of Tcf3, Lef1 or Tcf1-DN did not support ES cells to self-renew. Ectopic expression of either Lef1 or Lef1-DN blocked neuronal differentiation, suggesting that the transient induction of Lef1 was necessary for the initiation and progress of differentiation. ChIP analysis shows that Tcf1 bound to Nanog promoter and ectopic expression of Tcf1 enhanced the transcription of Nanog.
Conclusions
The overall data suggest that Tcf1 plays a critical role in the maintenance of stemness whereas Lef1 is involved in the initiation of differentiation.
5.Accumulation and Aberrant Modifications of alpha-Crystallins in Anterior Polar Cataracts.
Kyung Hoon HWANG ; Eunjoo H LEE ; Eek Hoon JHO ; Jae Ho KIM ; Do Hyung LEE ; Sung Kun CHUNG ; Eung Kwon KIM ; Choun Ki JOO
Yonsei Medical Journal 2004;45(1):73-80
Crystallins are the major proteins found in the lens, and the localization of specific crystallins is well known. Overexpression and accumulation of alphaB-crystallin has been observed in response to stress conditions or in certain diseases, such as brain tumors and neurodegenerative diseases. The purpose of this study was to examine whether alpha-crystallins are modified during pathological myofibroblastic changes in lens epithelial cells. Lens epithelial cells attached to the anterior capsules of patients with nuclear or anterior polar cataracts were analyzed quantitatively for alpha-crystallin proteins and mRNAs using Western blot and RT-PCR analysis., respectively. The degree of modification of alpha-crystallins was determined by 2-dimensional gel electrophoresis followed by Western blotting. Higher molecular weight protein bands that were immunoreactive to anti-alphaA- and anti-alphaB-crystallin antibodies around 45 kDa accumulated more in the anterior polar cataract samples than in those with the nuclear type of cataracts. Also monomeric alphaB-crystallins accumulated more in lens epithelial cells of patients with anterior polar cataracts. By comparison, no significant changes were found in the levels of the mRNAs encoding alphaA- and alphaB-crystallins in the different types of cataracts. Both alphaA- and alphaB-crystallin proteins seemed to undergo more extensive modification in anterior polar cataracts. Conclusion. In addition to fibrotic changes, which accompany increased levels of extracellular matrix molecules, accumulation and abnormal modification of alpha-crystallins might be implicated in the pathogenic mechanism of this type of cataract.
Adult
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Cataract/*genetics/metabolism
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Epithelial Cells/metabolism
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Female
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Human
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Lens, Crystalline/metabolism
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Male
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Middle Aged
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RNA, Messenger/analysis
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Reverse Transcriptase Polymerase Chain Reaction
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Support, Non-U.S. Gov't
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alpha-Crystallin A Chain/*genetics/metabolism
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alpha-Crystallin B Chain/*genetics/metabolism