Transcriptional Rates of Granulocyte-Macrophage Colony-Stimulating Factor, Granulocyte Colony-Stimulating Factor, Interleukin-3, and Macrophage Colony-Stimulating Factor Genes in Activated Cord Versus Adult Mononuclear Cells: Alteration in Cytokine Expression May Be Secondary to Posttranscriptional Instability

Sun Min Lee; Eva Knoppel; Carmella Van De Yen; Mitchell S Cairo

摘要

We have previously demonstrated that protein production and mRNA expression of granulocyte-macrophage colony-stimulating factor (GM-CSF), granulocyte colony-stimulating factor (G-CSF), and IL-3 are decreased in activated mononuclear cells (MNC) from human umbilical cord compared with adult peripheral blood. Reduced production of these colony-stimulating factors (CSF) during states of increased demand, as occurs during overwhelming bacterial infection, may play a role in the pathogenesis of ncutropenia and thrombocytopenia in the newborn. To determine whether the reduced mRNA expression and CSF production from activated cord MNC is secondary to the decreased transcriptional activity of the corresponding genes, we determined the transcriptional rate of GM-CSF, G-CSF, IL-3, and M-CSF by nuclear run-on assays. Cord and adult MNC were isolated by Ficoll-Hypaque density centrifugation. A total of 108 MNC from cord and adult blood were stimulated as follows: GM-CSF and G-CSF [32 nmol/L phorbol-12-myristate-6-acetate (20 μg/L) + 2 mg/L phytohemagglutinin for 6 h]; IL-3 [32 nmol/L phorbol-12-myristate-6-acctate (20 μg/L) + 0.5 μmol/L A 23187 for 6 h]; and macrophage CSF (2 μg/ L recombinant human GM-CSF for 24 h). The nuclei from unstimulated and stimulated cells were isolated and labeled with 32P-uridine triphosphate. Newly elongated 32P-labeled RNA transcripts were hybridized to slot blots of CSF DNA. To minimize cross hybridization artifacts, short fragments (0.5–1.0 kb) of cDNA were used. The transcriptional rate increase of GM-CSF, G-CSF, IL-3, and macrophage CSF upon stimulation appears to be similar in both cord and adult MNC [GM-CSF: 260 ± 62% (cord) versus 270 ± 33% (adult); G-CSF: 220 ± 71 % (cord) versus 220 ± 44% (adult); IL-3: 150 ± 25% (cord) versus 160 ± 38% (adult); macrophage CSF: 130 ± 10% (cord) versus 150 ± 15% (adult), mean ± SD]. These findings indicate that cord MNC transcribe these CSF genes at the same level as adult MNC during states of increased demand (stimulation). Therefore, the decrease in CSF“ mRNA expression in activated cord versus adult MNC is probably not secondary to defects in transcriptional regulation. Alteration in posttranscriptional events, such as dysregulation of mRNA stability, could account for the difference between newborn and adult CSF expression.

机译：先前我们已经证明，在人类激活的单核细胞（MNC）中，粒细胞-巨噬细胞集落刺激因子（GM-CSF），粒细胞集落刺激因子（G-CSF）和IL-3的蛋白质产生和mRNA表达降低脐带与成人外周血相比。在需求旺盛的细菌感染期间，在需求增加的状态下，这些集落刺激因子（CSF）的产量降低可能在新生儿神经减少症和血小板减少症的发病机理中起作用。为了确定从激活的脐带MNC减少的mRNA表达和CSF产生是否是相应基因的转录活性降低的次要原因，我们通过核转录因子测定了GM-CSF，G-CSF，IL-3和M-CSF的转录速率连续测定。通过Ficoll-Hypaque密度离心分离脐带和成年MNC。分别刺激了来自脐带血和成人血液的108个MNC：GM-CSF和G-CSF [32 nmol / L phorbol-12-肉豆蔻酸酯-6-乙酸盐（20μg/ L）+ 2 mg / L植物血凝素6 H]; IL-3 [32 nmol / L佛波醇12-肉豆蔻酸酯-6-乙酸盐（20μg/ L）+ 0.5μmol/ L A 23187 6小时];和巨噬细胞CSF（2μg/ L重组人GM-CSF，持续24 h）。分离来自未刺激和刺激的细胞的细胞核，并用32P-尿苷三磷酸标记。将新拉长的32P标记的RNA转录本与CSF DNA的缝隙印迹杂交。为了最大程度地减少交叉杂交伪像，使用了cDNA的短片段（0.5–1.0 kb）。脊髓和成人MNC刺激后GM-CSF，G-CSF，IL-3和巨噬细胞CSF的转录速率增加似乎相似[GM-CSF：260±62 ％（绳）与270±33 ％（成人）; G-CSF：220±71 ％（绳索）对220±44 ％（成人）; IL-3：150±25 ％（绳索）对160±38 ％（成人）;巨噬细胞CSF：130±10 ％（绳索）与150±15 ％（成人），平均值±SD]。这些发现表明，在需求增加（刺激）的状态下，脐带MNC以与成年MNC相同的水平转录这些CSF基因。因此，与成人MNC相比，活化的脐带中CSF” mRNA表达的下降可能不是转录调控缺陷引起的。转录后事件的改变，例如mRNA稳定性的失调，可以解释新生儿和成人CSF表达之间的差异。

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