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Validation of an air/liquid interface device for TiO2 nanoparticle toxicity assessment on NR8383 cells: preliminary results

机译:对NR8383细胞TiO2纳米粒子毒性评估的空气/液面界面装置的验证:初步结果

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Investigations on adverse biological effects of nanoparticles (NP) are performed usually either in vivo on rodents or in vitro under submerged conditions where NP are in suspension into cell culture media. However, sedimentation of NP in vitro is a continuous process and to assess the exact deposited cellular dose remains difficult, as the cellular internal dose is a function of time. Moreover, the cellular responses to NP under submerged culture conditions or by exposing rodents by nose-only to NP aerosols might differ from those observed at physiological settings at the air-liquid interface (ALI). Rat alveolar NR8383 macrophages were exposed to aerosols at the air-liquid interface. We studied TiO2 NM105, a mixture of anatase and rutile. NR8383 cells were exposed to a single dose of 3.0 cm(2)/cm(2) of TiO2 aerosol. Following RNA extraction. transcriptome allowing full coverage of the rat genome was performed, and differentially expressed genes were retrieved. Their products were analyzed for functions and interaction with String DB. Only 126 genes were differentially expressed and 98 were recognized by String DB and give us the gene expression signature of exposed rat alveolar NR8383 macrophages. Among them, 13 display relationships at a high confidence level and the ten most differentially expressed compared to unexposed cells were: Chad1, Ccl4, Zfp668, Fam129b, Nab2, Txnip, Id1, Cdc42ep3, Dusp6 and Myc, ranked from the most overexpressed to the most under-expressed. Some of them were previously described as over or under-expressed in NP exposed cell systems. We validated in our laboratory an easy-to-use device and a physiological relevant paradigm for studying the effects of cell exposure to TiO2. Ccl4 gene expression seems to be a positive marker of exposure evidenced as well as in vivo or in both in vitro conditions.
机译:关于纳米颗粒(NP)不良生物效应的研究通常在啮齿类动物体内进行,或在将NP悬浮在细胞培养基中的浸没条件下进行体外研究。然而,NP在体外的沉积是一个连续的过程,由于细胞内剂量是时间的函数,因此很难评估准确的沉积细胞剂量。此外,在浸没培养条件下或仅通过鼻子将啮齿类动物暴露于NP气溶胶中,细胞对NP的反应可能与在气液界面(ALI)的生理环境下观察到的反应不同。大鼠肺泡NR8383巨噬细胞暴露于气液界面的气溶胶中。我们研究了锐钛矿和金红石的混合物TiO2 NM105。NR8383细胞暴露于单剂量3.0 cm(2)/cm(2)的TiO2气溶胶中。RNA提取后。对大鼠基因组进行转录组全覆盖,并检索差异表达基因。对他们的产品进行了功能分析,并与字符串数据库进行了交互。只有126个基因被差异表达,98个基因被String DB识别,为我们提供了暴露的大鼠肺泡NR8383巨噬细胞的基因表达特征。其中有13种高置信度的显示关系,与未暴露细胞相比,10种表达差异最大的细胞是:Chad1、Ccl4、Zfp668、Fam129b、Nab2、Txnip、Id1、Cdc42ep3、Dusp6和Myc,从最高表达到最低表达排列。其中一些之前被描述为在NP暴露的细胞系统中过度表达或表达不足。我们在实验室中验证了一种易于使用的设备和一种生理学相关范式,用于研究细胞暴露于TiO2的影响。Ccl4基因的表达似乎是暴露的积极标志,无论是在体内还是在体外条件下都有证据证明。

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