Koo S H, Cunningham M C, Arabshahi B, Gruss J S, Grant J H
Department of Plastic and Reconstructive Surgery, Korea University, Seoul.
Plast Reconstr Surg. 2001 Sep 15;108(4):938-48; discussion 949-51. doi: 10.1097/00006534-200109150-00018.
The recent report of a transforming growth factor-beta 3 (TGF-beta 3) knock-out mouse in which 100 percent of the homozygous pups have cleft palate raised the question as to the potential usefulness of these animals as a model for cleft palate research. The specific aim in this study was to carefully document the anatomy of the cleft palate in the TGF-beta 3 knock-out mice as compared with wild type controls. Special attention was paid to the levator veli palatini muscle, the tensor veli palatini muscle, and their respective innervation. Because the TGF-beta 3 knock-out is lethal in the early perinatal period and because the heterozygotes are phenotypically normal, polymerase chain reaction was required to genotype the animals before mating. Time-mated pregnancies between proven heterozygotes were then delivered by cesarean section at gestational day 18.5 to prevent maternal cannibalism of homozygote pups. All delivered pups were killed and their tails processed by polymerase chain reaction to verify genotype. The heads were then fixed and sectioned in axial, coronal, or sagittal planes. Sections were stained with hematoxylin and eosin or processed for immunohistochemistry with nerve specific protein gene product 9.5 and calcitonin gene-related peptide antibodies. Sections were analyzed in a serial fashion. Nine wild type control animals were analyzed along with nine TGF-beta 3 knock-out homozygotes. Time matings between proven heterozygotes yielded wild type pups, heterozygote pups, and homozygote knock-out pups in the expected mendelian ratios (28 percent to 46 percent to 26 percent; n = 43). The results demonstrated 100 percent clefting in the homozygous TGF-beta 3 knock-out pups. Complete clefting of the secondary palate was seen in four of nine and incomplete clefting was seen in five of nine. The levator veli palatini and tensor veli palatini muscles were demonstrated coursing parallel to the cleft margin in all cleft mice. The orientation of these muscles differs from the normal transverse sling of the levator veli palatini muscle and the normal palatine aponeurosis of the tensor veli palatini muscle at the soft palate in control animals. Innervation of the levator veli palatini muscle by cranial nerve IX and the tensor veli palatini muscle by cranial nerve V were demonstrated in both cleft and control animals by use of immunohistochemistry with nerve-specific antibodies. Demonstration of a teratogen-free, reproducible animal model of clefting of the palate with a known, single-gene etiology is an important step in the systematic understanding of a congenital defect whose multifactorial etiology has hampered previous research efforts. This study presents a detailed anatomic description of such a model, including a description of the muscular anatomy and the innervation of the muscles of the palate. Because of early perinatal mortality, this model has limited applications for postnatal studies.
最近有关于转化生长因子β3(TGF-β3)基因敲除小鼠的报道,其中100%的纯合子幼崽患有腭裂,这引发了关于这些动物作为腭裂研究模型的潜在实用性的问题。本研究的具体目的是仔细记录与野生型对照相比,TGF-β3基因敲除小鼠腭裂的解剖结构。特别关注腭帆提肌、腭帆张肌及其各自的神经支配。由于TGF-β3基因敲除在围产期早期是致死性的,且杂合子在表型上是正常的,因此在交配前需要通过聚合酶链反应对动物进行基因分型。然后在妊娠第18.5天通过剖宫产分娩经证实的杂合子之间的定时交配妊娠,以防止母鼠吃掉纯合子幼崽。所有分娩的幼崽均被处死,其尾巴通过聚合酶链反应处理以验证基因型。然后将头部固定并在轴向、冠状或矢状平面上切片。切片用苏木精和伊红染色或用神经特异性蛋白基因产物9.5和降钙素基因相关肽抗体进行免疫组织化学处理。对切片进行连续分析。分析了9只野生型对照动物和9只TGF-β3基因敲除纯合子。经证实的杂合子之间的定时交配产生了野生型幼崽、杂合子幼崽和纯合子基因敲除幼崽,其比例符合预期的孟德尔比率(28%至46%至26%;n = 43)。结果表明,纯合子TGF-β3基因敲除幼崽腭裂发生率为100%。9只中有4只出现完全性继发腭裂,5只出现不完全性腭裂。在所有腭裂小鼠中,腭帆提肌和腭帆张肌均显示与腭裂边缘平行走行。这些肌肉的方向与对照动物软腭处腭帆提肌的正常横向吊带和腭帆张肌的正常腭腱膜不同。通过使用神经特异性抗体进行免疫组织化学,在腭裂和对照动物中均证实了腭帆提肌由第九颅神经支配,腭帆张肌由第五颅神经支配。证明一种无致畸剂、可重复的腭裂动物模型,其病因是已知的单基因,这是系统理解一种先天性缺陷的重要一步,该缺陷的多因素病因阻碍了先前的研究工作。本研究提供了这种模型的详细解剖学描述,包括腭部肌肉解剖结构和肌肉神经支配的描述。由于围产期早期死亡率较高,该模型在出生后研究中的应用有限。
