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小鼠磨牙发育过程中釉原蛋白异构体时空表达模式的鉴定

Identification of temporal and spatial expression patterns of amelogenin isoforms during mouse molar development.

作者信息

Iacob Stanca, Veis Arthur

机构信息

Northwestern University, Feinberg School of Medicine, Department of Cell and Molecular Biology, Chicago, IL 60611, USA.

出版信息

Eur J Oral Sci. 2006 May;114 Suppl 1:194-200; discussion 201-2, 381. doi: 10.1111/j.1600-0722.2006.00287.x.

DOI:10.1111/j.1600-0722.2006.00287.x
PMID:16674685
Abstract

Amelogenin synthesis is initiated in a restricted time frame during odontogenesis. Polypeptides translated from several alternatively spliced isoforms of amelogenin mRNA have been identified in ameloblasts and odontoblasts. Recent studies suggest that the isoforms deleting exons 6a, 6b, and 6c produce polypeptides that might exert regulatory functions governing the late stages of ameloblast and odontoblast differentiation. Herein, the spatial and temporal expression of mouse amelogenin mRNA isoforms M194, M180, M73, and M59 have been determined around the perinatal development period using splice form-specific probes. Expression levels and distribution patterns varied with developmental stage and cell location. Amelogenin mRNA expression was most prominent within the enamel organ at boundaries between cell layers, beginning at the newborn stage (PN0.5). Odontoblasts supported the expression of M73 and M59 mRNA from developmental stages PN0.5 to PN1.5 (1 d of age). In contrast, ameloblasts expressed predominantly the M180 mRNA isoform with full exon 6 but devoid of exon 4. In the enamel organ, the stratum intermediun cells supported expression of the full-length isoform, M194, including the full exon 6 and exon 4 sequences, and strikingly, expression of M180 message was inhibited. In conclusion, ameloblasts, odontoblasts, and stratum intermedium cells demonstrate selective alternative splicing patterns of the amelogenin pre-mRNA transcript.

摘要

釉原蛋白的合成在牙胚发生过程中的特定时间范围内启动。在成釉细胞和成牙本质细胞中已鉴定出从釉原蛋白mRNA的几种可变剪接异构体翻译而来的多肽。最近的研究表明,缺失外显子6a、6b和6c的异构体产生的多肽可能发挥调控成釉细胞和成牙本质细胞分化后期的功能。在此,使用剪接形式特异性探针确定了小鼠釉原蛋白mRNA异构体M194、M180、M73和M59在围产期发育期间的时空表达。表达水平和分布模式随发育阶段和细胞位置而变化。从新生阶段(出生后0.5天)开始,釉原蛋白mRNA表达在釉器细胞层之间的边界处最为突出。从发育阶段出生后0.5天到出生后1.5天(1日龄),成牙本质细胞支持M73和M59 mRNA的表达。相反,成釉细胞主要表达具有完整外显子6但缺失外显子4的M180 mRNA异构体。在釉器中,中间层细胞支持全长异构体M194的表达,包括完整的外显子6和外显子4序列,并且引人注目的是,M180 mRNA的表达受到抑制。总之,成釉细胞、成牙本质细胞和中间层细胞表现出釉原蛋白前体mRNA转录本的选择性可变剪接模式。

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