2016
DOI: 10.1080/15548627.2016.1196313
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Upregulation of SQSTM1/p62 contributes to nickel-induced malignant transformation of human bronchial epithelial cells

Abstract: Chronic lung inflammation is accepted as being associated with the development of lung cancer caused by nickel exposure. Therefore, identifying the molecular mechanisms that lead to a nickel-induced sustained inflammatory microenvironment that causes transformation of human bronchial epithelial cells is of high significance. In the current studies, we identified SQSTM1/p62 as a novel nickel-upregulated protein that is important for nickel-induced inflammatory TNF expression, subsequently resulting in transform… Show more

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Cited by 73 publications
(55 citation statements)
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“…The effect of MEG3 on the expression of c-Jun and c-Myc was further validated in Beas2B(shMEG3) cells(Figure 5F). These results are also consistent with our most recently findings that nickel exposure leads to a marked nuclear translocation of c-Jun and c-Myc 26 . Therefore, we proposed that c-Jun and c-Myc might be the transcription factors for negative regulation of phlpp1 promoter transactivation through direct binding.…”
Section: Resultssupporting
confidence: 93%
“…The effect of MEG3 on the expression of c-Jun and c-Myc was further validated in Beas2B(shMEG3) cells(Figure 5F). These results are also consistent with our most recently findings that nickel exposure leads to a marked nuclear translocation of c-Jun and c-Myc 26 . Therefore, we proposed that c-Jun and c-Myc might be the transcription factors for negative regulation of phlpp1 promoter transactivation through direct binding.…”
Section: Resultssupporting
confidence: 93%
“…An NF-kB response element has been identified in the p62 promoter (Vadlamudi & Shin, 1998). Our work showed, in agreement with previous studies (Huang et al, 2016), that NF-kB/p65 binds p62 promoter and plays an important role for p62 transcriptional regulation.…”
Section: Discussionsupporting
confidence: 92%
“…The primers used in this study were: human mmp‐2 (Forward: 5′‐caa gtg gga caa gaa cca ga‐3′, Reverse: 5′‐cca aag ttg atc atg atg tc‐3′), human sp1 (Forward: 5′‐att aac ctc agt gca ttg ggt a‐3′, Reverse: 5′‐agg gca ggc aaa ttt ctt ctc‐3′), human jnk2 (Forward: 5′‐atg aag aaa ctt cag cca act gt‐3′, Reverse: 5′‐aca gat ctc tgg ctt gac tt ‐3′) and human gapdh (Forward: 5′‐gat gat ctt gag gct gtt gtc‐3′, Reverse: 5′‐cag ggc tgc ttt taa ctc tg‐3′). Real‐time PCR was conducted following the protocol for Fast SYBR Green Master Mix kit (Applied Biosystems, Foster City, CA, USA; 4385614) in the 7900HT Fast Real‐Time PCR System (Applied Biosystems) using the same cDNs used for RT‐PCR as described in our previous publication (Huang et al ., ).…”
Section: Methodsmentioning
confidence: 97%