破骨细胞中plectin亚型的表达分析

T. Matsubara, Mariko Urata, W. Addison, S. Kokabu
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To reveal the roles of Plectin in osteoclasts, we examined the expression levels of Plectin isoforms and found the isoforms regulating actin organization are highly expressed in osteoclasts. *Correspondence to: Takuma Matsubara, Division of Molecular Signaling and Biochemistry, Department of Health Improvement, Kyushu Dental University, 2-6-1, Manazuru, Kitakyushu, Fukuoka, 8038580, Japan, Tel: +81-93-285-3049, Fax: +81-93-582-6000, E-mail: r15matsubara@fa.kyu-dent.ac.jp Received: February 01, 2019; Accepted: February 15, 2019; Published: February 18, 2019 Introduction Osteoclasts are one of the major player for bone resorption and regulate bone remodeling to maintain bone homeostasis [1,2]. Activation of osteoclastic bone resorption in comparison with bone formation by osteoblasts results in bone metabolic diseases such as osteoporosis and periodontal disease [3-5]. Moreover, the function of osteoclasts is important in orthodontic treatments, oral implant treatment and pathogenesis of osteonecrosis of the jaw [6-9]. Thus, regulation of osteoclasts is one of the serious themes for improvement of various dental treatments. Osteoclasts are differentiated from hematopoietic stem cells with macrophage colony stimulating factor (M-CSF) and Receptor activator NF-κB ligand (RANKL) stimulation [1,2]. Attachment and sealing of bone matrix by differentiated osteoclasts is essential for bone resorption [10,11]. Actin, tubulin and intermediate filaments are dynamically organized and forms actin ring that is consistent with actin dots called podosomes in cell periphery for attachment and sealing [12-15]. It is well known that the mice defect actin ring formation by knocking out a tyrosine kinase Src are osteopetrosis because of decrease of bone resorbing activity [16,17]. This indicates Src is one of the key molecules to regulate bone resorption. We identified a cytolinker protein Plectin as a partner of Src and organize actin ring formation in osteoclasts [13]. Plectin was highly expressed in brain, heart, skeletal muscle and TRAP(+) MNCs [13,14,18,19]. Plectin has 13 isoforms and there role is a little different each other [18]. This suggests Plectin variants plays different roles in each tissue. Here, we explore the important isoforms of Plectin in osteoclasts. Materials and methods Animals 4 weeks old C57BL6/N mice were purchased from Japan SLC, Inc. (Shizuoka, Japan). Spleen and femoral muscle were obtained from these mice. Spleen cells were differentiated to osteoclast like cells with M-CSF and sRANKL described as previously [13,15]. Femoral muscle was mashed with Biomasher II purchased from Nippi (Tokyo, Japan) and obtained mRNA described below. Real-time quantitative PCR Total RNA of the biceps muscle of the thigh, spleen cell derived osteoclasts as described previously [15]. rRNAs were isolated with FastGeneTM RNA Basic Kit from Nippon genetics Co., ltd. (Tokyo, Japan). cDNA was synthesized from 1 μg of total RNA by using ReverTra Ace from TOYOBO (Tokyo, Japan). Real-time quantitative PCR was performed by incubating cDNA, PowerUp SYBRTM Green Master Mix from Thermo Fisher Scientific and primers indicated at below in a QuantStudio 3 Real-time PCR system purchased from Thermo Fisher Scientific (San Jose, CA). All reactions were performed in triplicate and analyzed. The expression level was normalized by Gapdh expression. The primer sequences were: Gapdh, 5′-aactttggcattgtggaagg-3′ (forward) and 5′-acacattggggtaggaaca-3′ (reverse); Plec1, 5′-ggagcctgccccagccacag-3′ (forward); Plec1a, 5′-gggcaagaaagatgaacgag-3′ (forward); Plec1b, 5′cggcaggcaaaggatgagcaag-3′ (forward); Plec1c, 5′ggccgtcatccgcattgcag-3′ (forward); Plec1d, 5′ccccaatgaagatcgtgcccg-3′ (forward); Plec1e, 5′agcacgagatcagctccctcaaag-3′ (forward); Plec1f, 5′aggaggtgcgggagaagtacaaag-3′ (forward); Plec1g, 5′ctctacgggcaactctgttgtgtag-3′ (forward); Plec1hij, 5′atgaacgagaccgtgtgcagaag-3′ (forward); Plec1 common, 5′cctgagaggacttccagcag-3′ (reverse); Src, 5′gttgcttcggagaggtgtggat-3′ (forward) and 5′caccagtttctcgtgcctcagt-3′ (reverse). The experiments were individually performed at least twice and obtained representative data. Data analysis and statistics The experiments were performed at least twice. Differences between groups were analyzed by the Student’s t-test to determine statistical significance. 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Individual Plectin isoforms have different roles. To reveal the roles of Plectin in osteoclasts, we examined the expression levels of Plectin isoforms and found the isoforms regulating actin organization are highly expressed in osteoclasts. *Correspondence to: Takuma Matsubara, Division of Molecular Signaling and Biochemistry, Department of Health Improvement, Kyushu Dental University, 2-6-1, Manazuru, Kitakyushu, Fukuoka, 8038580, Japan, Tel: +81-93-285-3049, Fax: +81-93-582-6000, E-mail: r15matsubara@fa.kyu-dent.ac.jp Received: February 01, 2019; Accepted: February 15, 2019; Published: February 18, 2019 Introduction Osteoclasts are one of the major player for bone resorption and regulate bone remodeling to maintain bone homeostasis [1,2]. Activation of osteoclastic bone resorption in comparison with bone formation by osteoblasts results in bone metabolic diseases such as osteoporosis and periodontal disease [3-5]. Moreover, the function of osteoclasts is important in orthodontic treatments, oral implant treatment and pathogenesis of osteonecrosis of the jaw [6-9]. Thus, regulation of osteoclasts is one of the serious themes for improvement of various dental treatments. Osteoclasts are differentiated from hematopoietic stem cells with macrophage colony stimulating factor (M-CSF) and Receptor activator NF-κB ligand (RANKL) stimulation [1,2]. Attachment and sealing of bone matrix by differentiated osteoclasts is essential for bone resorption [10,11]. Actin, tubulin and intermediate filaments are dynamically organized and forms actin ring that is consistent with actin dots called podosomes in cell periphery for attachment and sealing [12-15]. It is well known that the mice defect actin ring formation by knocking out a tyrosine kinase Src are osteopetrosis because of decrease of bone resorbing activity [16,17]. This indicates Src is one of the key molecules to regulate bone resorption. 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引用次数: 0

摘要

为了探索破骨细胞中表达的同种异构体,我们与骨骼肌进行了实时定量PCR分析,其中同种异构体起作用[20](图1)。TRAP(+)跨国公司中Plectin 1、1b、1d、1e、1f和1g的表达水平高于骨骼肌(图1)。由于引物设计,Plectin 1h、1i和1j没有相互区分。另一方面,在TRAP(+)跨国公司中,Plectin 1a和1c较少。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Expression analysis of plectin isoforms in osteoclast
Bone homeostasis is maintained by osteoclasts and osteoblasts. Regulation of bone homeostasis is important for orthodontic treatments, oral implant, treatment for periodontal disease, osteonecrosis of the jaw and so on. We reported an intermediate filament linking protein Plectin plays important role in osteoclastic bone resorption. Plectin is a large molecule >500 kDa and have 13 isoforms. Individual Plectin isoforms have different roles. To reveal the roles of Plectin in osteoclasts, we examined the expression levels of Plectin isoforms and found the isoforms regulating actin organization are highly expressed in osteoclasts. *Correspondence to: Takuma Matsubara, Division of Molecular Signaling and Biochemistry, Department of Health Improvement, Kyushu Dental University, 2-6-1, Manazuru, Kitakyushu, Fukuoka, 8038580, Japan, Tel: +81-93-285-3049, Fax: +81-93-582-6000, E-mail: r15matsubara@fa.kyu-dent.ac.jp Received: February 01, 2019; Accepted: February 15, 2019; Published: February 18, 2019 Introduction Osteoclasts are one of the major player for bone resorption and regulate bone remodeling to maintain bone homeostasis [1,2]. Activation of osteoclastic bone resorption in comparison with bone formation by osteoblasts results in bone metabolic diseases such as osteoporosis and periodontal disease [3-5]. Moreover, the function of osteoclasts is important in orthodontic treatments, oral implant treatment and pathogenesis of osteonecrosis of the jaw [6-9]. Thus, regulation of osteoclasts is one of the serious themes for improvement of various dental treatments. Osteoclasts are differentiated from hematopoietic stem cells with macrophage colony stimulating factor (M-CSF) and Receptor activator NF-κB ligand (RANKL) stimulation [1,2]. Attachment and sealing of bone matrix by differentiated osteoclasts is essential for bone resorption [10,11]. Actin, tubulin and intermediate filaments are dynamically organized and forms actin ring that is consistent with actin dots called podosomes in cell periphery for attachment and sealing [12-15]. It is well known that the mice defect actin ring formation by knocking out a tyrosine kinase Src are osteopetrosis because of decrease of bone resorbing activity [16,17]. This indicates Src is one of the key molecules to regulate bone resorption. We identified a cytolinker protein Plectin as a partner of Src and organize actin ring formation in osteoclasts [13]. Plectin was highly expressed in brain, heart, skeletal muscle and TRAP(+) MNCs [13,14,18,19]. Plectin has 13 isoforms and there role is a little different each other [18]. This suggests Plectin variants plays different roles in each tissue. Here, we explore the important isoforms of Plectin in osteoclasts. Materials and methods Animals 4 weeks old C57BL6/N mice were purchased from Japan SLC, Inc. (Shizuoka, Japan). Spleen and femoral muscle were obtained from these mice. Spleen cells were differentiated to osteoclast like cells with M-CSF and sRANKL described as previously [13,15]. Femoral muscle was mashed with Biomasher II purchased from Nippi (Tokyo, Japan) and obtained mRNA described below. Real-time quantitative PCR Total RNA of the biceps muscle of the thigh, spleen cell derived osteoclasts as described previously [15]. rRNAs were isolated with FastGeneTM RNA Basic Kit from Nippon genetics Co., ltd. (Tokyo, Japan). cDNA was synthesized from 1 μg of total RNA by using ReverTra Ace from TOYOBO (Tokyo, Japan). Real-time quantitative PCR was performed by incubating cDNA, PowerUp SYBRTM Green Master Mix from Thermo Fisher Scientific and primers indicated at below in a QuantStudio 3 Real-time PCR system purchased from Thermo Fisher Scientific (San Jose, CA). All reactions were performed in triplicate and analyzed. The expression level was normalized by Gapdh expression. The primer sequences were: Gapdh, 5′-aactttggcattgtggaagg-3′ (forward) and 5′-acacattggggtaggaaca-3′ (reverse); Plec1, 5′-ggagcctgccccagccacag-3′ (forward); Plec1a, 5′-gggcaagaaagatgaacgag-3′ (forward); Plec1b, 5′cggcaggcaaaggatgagcaag-3′ (forward); Plec1c, 5′ggccgtcatccgcattgcag-3′ (forward); Plec1d, 5′ccccaatgaagatcgtgcccg-3′ (forward); Plec1e, 5′agcacgagatcagctccctcaaag-3′ (forward); Plec1f, 5′aggaggtgcgggagaagtacaaag-3′ (forward); Plec1g, 5′ctctacgggcaactctgttgtgtag-3′ (forward); Plec1hij, 5′atgaacgagaccgtgtgcagaag-3′ (forward); Plec1 common, 5′cctgagaggacttccagcag-3′ (reverse); Src, 5′gttgcttcggagaggtgtggat-3′ (forward) and 5′caccagtttctcgtgcctcagt-3′ (reverse). The experiments were individually performed at least twice and obtained representative data. Data analysis and statistics The experiments were performed at least twice. Differences between groups were analyzed by the Student’s t-test to determine statistical significance. A value of P < 0.01 was considered statistically significant. Matsubara T (2019) Expression analysis of plectin isoforms in osteoclast Dent Oral Craniofac Res, 2019 doi: 10.15761/DOCR.1000286 Volume 5: 2-3 Results To explore what isoform is expressed in osteoclasts, we performed real-time quantitative PCR analysis compared with skeletal muscle where what isoform is working [20] (Figure 1). Expression level of Plectin 1, 1b, 1d, 1e, 1f and 1g in TRAP(+) MNCs was higher than in skeletal muscle (Figure 1). Plectin 1h, 1i and 1j were not distinguished each other due to primer design. On the other hand, Plectin 1a and 1c were less in TRAP (+) MNCs.
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