体外胚胎培养和胚胎移植产生的小鼠胎儿肺组织中 Toll-Like 受体的表达。

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-01-01 Epub Date: 2023-04-27 DOI:10.1159/000529974
Göksel Doğan, Nedim Karagenç, Kerem Esmen, Bengi Çınar Kul, Hasan Yeşilkaya, Şakir Akgün, Mehmet Nurullah Orman, Mustafa Sandıkçı, Ülker Eren, Hümeyra Ünsal, Levent Karagenç
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引用次数: 0

摘要

通过体外胚胎培养和胚胎移植产生的小鼠胎儿表现出肺发育受损、肺上皮细胞组成改变以及与肺发育和TLR信号通路相关的多个基因下调。本研究的目的是确定所有 TLR 的表达,并研究通过胚胎培养和胚胎移植产生的小鼠胎儿的肺组织中 TLR 的表达以及参与 TLR 信号通路的基因是否发生了改变。研究包括两个实验组(EG)和一个对照组(CG)。将在 5% CO2-95% 空气中培养 95 小时或不足 24 小时的胚胎移植到假孕雌鼠体内,分别获得体外 EG(18 个)和体内 EG(18 个)胎儿。自然排卵雌鼠在妊娠第 18 天获得的胎儿作为 CG(n = 18)。采用 Western 印迹法和免疫组化法测定 TLR 蛋白的表达。采用 qRT-PCR 方法测定了编码 TLRs 的转录本和参与 TLR 信号通路的基因(Lbp、Pik3r1、Pik3cb、Nfkbia 和 Fos)的表达。虽然所有组别的肺组织支气管/支气管上皮内衬细胞都表达了所有的 TLRs,但其中一些 TLRs 有特定的表达模式。与 CG 相比,编码 TLR-2、-3、-4、-5、-7、-8、-9、-12、-13、Lbp、Pik3r1、Pik3cb、Nfkbia 和 Fos 的转录物在两种 EG 中的表达均显著下调。看来,在胚胎植入前的发育阶段对胚胎施加的压力与围产期肺组织中 TLRs 以及参与 TLR 信号通路的一些基因的下调有关。至于 TLRs 以及参与 TLR 信号通路的基因的下调是否会对成年肺组织产生任何功能性影响,还有待确定。
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Expression of Toll-Like Receptors in the Lung Tissue of Mouse Fetuses Generated by in vitro Embryo Culture and Embryo Transfer.

Mouse fetuses generated by in vitro embryo culture and embryo transfer exhibit impaired lung development, altered composition of pulmonary epithelial cells associated with downregulation of several genes involved in lung development and toll-like receptor (TLR) signaling pathway. The aims of the present study were to determine the expression of all TLRs and to examine if the expression of TLRs, along with genes involved in TLR signaling pathway, is altered in the lung tissue of mouse fetuses generated through embryo culture and embryo transfer. Two experimental (EGs) and one control (CG) group were included in the study. Embryos cultured at 5% CO2-95% air for 95 h or less than 24 h were transferred to pseudo-pregnant females to obtain fetuses comprising EGin vitro (n = 18) and EGin vivo (n = 18), respectively. Fetuses obtained from naturally ovulating females on day 18 of pregnancy served as the CG (n = 18). Western blot and immunohistochemistry were used to determine the expression of TLR proteins. The expression of transcripts encoding TLRs, and the genes involved in TLR signaling pathway (Lbp, Pik3r1, Pik3cb, Nfkbia, and Fos), was determined using qRT-PCR. While all TLRs were expressed by cells lining the bronchial/bronchiolar epithelium of lung tissues in all groups, some of the TLRs were expressed in a specific pattern. When compared to CG, the expression of transcripts encoding TLR-2, -3, -4, -5, -7, -8, -9, -12, -13, Lbp, Pik3r1, Pik3cb, Nfkbia, and Fos was significantly downregulated in both EGs. It appears that stress imposed on embryos at preimplantation stages of development is associated with downregulation of TLRs, along with some of the genes involved in TLR signaling pathway, in the lung tissue during the perinatal period. It remains to be determined if downregulation of TLRs, along with the genes involved in TLR signaling pathway, has any functional consequences in the adult lung tissue.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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