STRUCTURE/FUNCTION OF SURFACTANT PROTEIN D

表面活性蛋白 D 的结构/功能

• 批准号: 6536967
• 负责人: ERIKA Christine CROUCH
• 金额: $ 31.11万
• 依托单位: BARNES-JEWISH HOSPITAL
• 依托单位国家: 美国
• 财政年份: 1990
• 资助国家: 美国
• 起止时间: 1990-01-01 至 2003-07-31
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/6536967
• 关键词: AP1 protein; cytokine; enhancer binding protein; gel mobility shift assay; gene expression; genetic mapping; genetic regulatory element; genetic transcription; glucocorticoids; glycoprotein structure; laboratory rat; lectin; polymerization; protein folding; protein purification; protein structure function; pulmonary surfactants; recombinant proteins; respiratory epithelium; tissue /cell culture; transfection

Surfactant Protein D (SP-D) is a collagenous carbohydrate binding protein that is secreted into the airspaces of the lung by type II and nonciliated bronchiolar epithelial cells. SP-D binds to glycoconjugates expressed on various microorganisms and particulate antigens, can modulate the activities of inflammatory cells, and may also contribute to the metabolism of lung surfactant. SP-D production increases following lung injury consistent with its participation in the pulmonary "acute phase response" (APR). For these reasons, it is important to understand the mechanisms that regulate the expression of SP-D and its accumulation in the airspace. Our studies have shown that the assembly of trimeric subunits and the formation of dodecamers or larger multimers is important- if not critical- for many of it's activities. In addition, our studies of the human gene have lead to the identification of a conserved AP-1 element (-109) and a functional C/EBP-like protein binding sequence (-340) that could contribute to basal expression and the increased expression of SP-D following lung injury. Accordingly. we propose four aims. First, we plan to further characterize the proximal promoter with emphasis on the conserved sequences that flank the AP-1 element, including a downstream HNF-3 binding site and an upstream binding site that includes overlapping E-Box, GT- box and GATA-like motifs. Second, we will further characterize the putative C/EBP element at -340 and a tandem motif at -319, and examine the contribution of other C/EBP motifs and potential STAT binding sequences. We will also examine potential modulatory effects of retinoblastoma protein and glucocorticoids on C/EBP- mediated transcriptional activation, and the regulatory activities of IL-6 and other cytokines and hormones previously implicated in the regulation of the hepatic APR. Third, we propose to characterize a recently identified untranslated exon within "intron 1" of the human gene. Fourth, we propose to continue with studies examining the mechanisms of SP-D trimerization, multimerization, and secretion of SP-D. Our ongoing and proposed studies will provide important information related to the regulation of SP-D production, the assembly of functional multimers, and the response of the lung to microbial challenge and other forms of lung injury.

表面活性蛋白D（SP-D）是一种胶原性碳水化合物结合蛋白，由II型和无纤毛的细支气管上皮细胞分泌到肺的气隙中。 SP-D与各种微生物和颗粒抗原上表达的糖缀合物结合，可以调节炎性细胞的活性，并且还可能有助于肺表面活性物质的代谢。 肺损伤后SP-D产生增加，与其参与肺“急性期反应”（APR）一致。 由于这些原因，重要的是要了解调节SP-D的表达及其在空气中的积累的机制。 我们的研究表明，三聚体亚基的组装和十二聚体或更大的多聚体的形成对于它的许多活动来说是重要的-如果不是关键的话。 此外，我们对人类基因的研究已经鉴定出保守的AP-1元件（-109）和功能性C/EBP样蛋白结合序列（-340），它们可能有助于肺损伤后SP-D的基础表达和表达增加。 相应地我们提出四个目标。 首先，我们计划进一步表征近端启动子，重点是AP-1元件侧翼的保守序列，包括下游HNF-3结合位点和上游结合位点，其包括重叠的E-Box、GT- box和GATA样基序。 第二，我们将进一步表征假定的C/EBP元件在-340和串联基序在-319，并检查其他C/EBP基序和潜在的STAT结合序列的贡献。 我们还将研究视网膜母细胞瘤蛋白和糖皮质激素对C/EBP介导的转录激活的潜在调节作用，以及IL-6和其他细胞因子和激素的调节活性，这些细胞因子和激素先前参与了肝脏APR的调节。第三，我们建议描述最近发现的人类基因“内含子1”内的非翻译外显子。 第四，我们建议继续研究SP-D三聚化、多聚化和分泌SP-D的机制。 我们正在进行的和拟议的研究将提供与SP-D生产调节、功能性多聚体组装以及肺对微生物挑战和其他形式肺损伤的反应相关的重要信息。