Medford Andrew R L, Douglas Samantha K, Godinho Sofia I H, Uppington Kay M, Armstrong Lynne, Gillespie Kathleen M, van Zyl Berendine, Tetley Terry D, Ibrahim Nassif B N, Millar Ann B
Department of Clinical Science at North Bristol, University of Bristol Paul O'Gorman Lifeline Centre, Southmead Hospital, Westbury-on-Trym, Bristol, UK.
Respir Res. 2009 Apr 9;10(1):27. doi: 10.1186/1465-9921-10-27.
The properties of vascular endothelial growth factor (VEGF) as a potent vascular permogen and mitogen have led to investigation of its potential role in lung injury. Alternate spliced VEGF transcript generates several isoforms with potentially differing functions. The purpose of this study was to determine VEGF isoform expression and source in normal and ARDS subjects and investigate the expression and regulation of VEGF isoforms by human alveolar type 2 (ATII) cells.
VEGF protein expression was assessed immunohistochemically in archival normal and ARDS human lung tissue. VEGF isoform mRNA expression was assessed in human and murine lung tissue. Purified ATII cells were cultured with proinflammatory cytokines prior to RNA extraction/cell supernatant sampling/proliferation assay.
VEGF was expressed on alveolar epithelium, vascular endothelium and alveolar macrophages in normal and ARDS human lung tissue. Increases in VEGF expression were detected in later ARDS in comparison to both normal subjects and early ARDS (p < 0.001). VEGF121, VEGF165 and VEGF189 isoform mRNA expression increased in later ARDS (p < 0.05). The ratio of soluble to cell-associated isoforms was lower in early ARDS than normal subjects and later ARDS and also in murine lung injury. ATII cells constitutionally produced VEGF165 and VEGF121 protein which was increased by LPS (p < 0.05). VEGF165 upregulated ATII cell proliferation (p < 0.001) that was inhibited by soluble VEGF receptor 1 (sflt) (p < 0.05).
These data demonstrate that changes in VEGF isoform expression occur in ARDS which may be related to their production by and mitogenic effect on ATII cells; with potentially significant clinical consequences.
血管内皮生长因子(VEGF)作为一种强大的血管通透因子和促有丝分裂原,其特性促使人们对其在肺损伤中的潜在作用进行研究。VEGF转录本的可变剪接产生了几种可能具有不同功能的异构体。本研究的目的是确定正常人和急性呼吸窘迫综合征(ARDS)患者中VEGF异构体的表达和来源,并研究人肺泡Ⅱ型(ATII)细胞对VEGF异构体的表达和调控。
采用免疫组织化学方法评估存档的正常人和ARDS患者肺组织中VEGF蛋白的表达。评估人和小鼠肺组织中VEGF异构体mRNA的表达。纯化的ATII细胞在RNA提取/细胞上清液采样/增殖测定前用促炎细胞因子培养。
在正常人和ARDS患者的肺组织中,VEGF在肺泡上皮、血管内皮和肺泡巨噬细胞上表达。与正常人和早期ARDS相比,晚期ARDS中VEGF表达增加(p<0.001)。晚期ARDS中VEGF121、VEGF165和VEGF189异构体mRNA表达增加(p<0.05)。早期ARDS中可溶性异构体与细胞相关异构体的比例低于正常人和晚期ARDS,在小鼠肺损伤中也是如此。ATII细胞组成性产生VEGF165和VEGF121蛋白,脂多糖可使其增加(p<0.05)。VEGF165上调ATII细胞增殖(p<0.001),可溶性VEGF受体1(sflt)可抑制其增殖(p<0.05)。
这些数据表明,ARDS中VEGF异构体表达发生变化,这可能与其由ATII细胞产生及其对ATII细胞的促有丝分裂作用有关;可能具有重大的临床意义。
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