INRA, UMR1313 Unité Génétique Animale et Biologie Intégrative, équipe «Lait, Génome & Santé» F-78350 Jouy-en-Josas, France.
J Dairy Sci. 2012 Oct;95(10):6130-44. doi: 10.3168/jds.2012-5604. Epub 2012 Aug 23.
Mastitis, an inflammation of the mammary gland, is the most costly infectious disease of dairy ruminants worldwide. Although it receives considerable attention, the early steps of the host response remain poorly defined. Here, we report a noninvasive method using milk fat globules (MFG) as a source of mammary RNA to follow the dynamics of the global transcriptional response of mammary epithelial cells (MEC) during the course of a bacterial infection. We first assessed that RNA isolated from MFG were representative of MEC RNA; we then evaluated whether MFG RNA could be used to monitor the MEC response to infection. Sufficiently high yields of good-quality RNA (RNA integrity numbers ranging between 6.7 and 8.7) were obtained from goat MFG for subsequent analyses. Contamination of MFG by macrophages and neutrophils, which can be trapped during creaming, was assessed and when using quantitative real-time PCR for cell-type specific markers, was shown to be weak enough (<8%) to affect MFG gene expression profiling. Using microarrays, we showed that RNA extracted from MFG and from mammary alveolar parenchyma shared approximately 90% of the highlighted probes corresponding in particular to genes encoding milk proteins (CSN, BLG, LALBA) and enzymes involved in milk fat synthesis and secretion (FASN, XDH, ADRP, SCD, and DGAT1). In addition, a gene involved in the acute-phase reaction, coding for the serum amyloid A3 (SAA3) protein, was found within the first 50 most highly expressed genes in a noninfectious context in both mammary alveolar parenchyma and MFG, strongly suggesting that SAA3 is expressed in MEC. We took advantage of this noninvasive RNA sampling to follow the early proinflammatory response of MEC during the course of a bacterial infection and showed that the levels of mRNA encoding SAA3 sharply increased at 24h postinfection. Taken together, our results demonstrate that MFG represent a unique source of MEC RNA to noninvasively sample sufficient amounts of high-quality RNA to assess the dynamics of MEC gene expression in vivo, especially during the first steps of infection, thereby paving the way for the discovery of early biomarkers for the control of intramammary infections. Furthermore, this noninvasive technique could be used to provide mammary transcriptomic data on a large scale, thus filling the gap between genomic and phenotypic data.
乳腺炎是乳腺的炎症,是世界范围内奶牛反刍动物中最昂贵的传染性疾病。尽管它受到了相当多的关注,但宿主反应的早期步骤仍未得到很好的定义。在这里,我们报告了一种使用乳脂肪球(MFG)作为乳腺 RNA 来源的非侵入性方法,以跟踪乳腺上皮细胞(MEC)在细菌感染过程中的整体转录反应的动态。我们首先评估了从 MFG 中分离出的 RNA 是 MEC RNA 的代表;然后评估了 MFG RNA 是否可用于监测 MEC 对感染的反应。从山羊 MFG 中获得了足够高产量的高质量 RNA(RNA 完整性数在 6.7 到 8.7 之间),可用于后续分析。评估了在奶油过程中可能被捕获的巨噬细胞和中性粒细胞对 MFG 的污染,并且当使用定量实时 PCR 进行细胞类型特异性标记物时,发现其污染程度很弱(<8%),不足以影响 MFG 基因表达谱。使用微阵列,我们表明从 MFG 和乳腺腺泡实质中提取的 RNA 共享大约 90%的突出探针,特别是对应于编码乳蛋白(CSN、BLG、LALBA)和参与乳脂肪合成和分泌的酶的基因(FASN、XDH、ADRP、SCD 和 DGAT1)。此外,在非传染性环境中,乳腺腺泡实质和 MFG 中的前 50 个表达最高的基因中都发现了一个与急性期反应相关的基因,编码血清淀粉样蛋白 A3(SAA3)蛋白,这强烈表明 SAA3 在 MEC 中表达。我们利用这种非侵入性的 RNA 采样来跟踪细菌感染过程中 MEC 的早期促炎反应,并表明感染后 24 小时 SAA3 编码 mRNA 的水平急剧增加。总之,我们的结果表明,MFG 是 MEC RNA 的独特来源,可以非侵入性地采样足够数量的高质量 RNA,以评估体内 MEC 基因表达的动态,特别是在感染的早期阶段,从而为控制乳腺炎的早期生物标志物的发现铺平了道路。此外,这种非侵入性技术可用于大规模提供乳腺转录组数据,从而填补基因组和表型数据之间的空白。
