Department of Ophthalmology, School of Medicine, Emory University, Atlanta, Georgia 30322, USA.
Invest Ophthalmol Vis Sci. 2013 Jul 30;54(7):5111-22. doi: 10.1167/iovs.13-12336.
A mouse mutation, tvrm148, was previously reported as resulting in retinal degeneration. Tvrm148 and Rpe65 map between markers D3Mit147 and D3Mit19 on a genetic map, but the physical map places RPE65 outside the markers. We asked if Rpe65 or perhaps another nearby gene is mutated and if the mutant reduced 11-cis-retinal levels. We studied the impact of the tvrm148 mutation on visual function, morphology, and retinoid levels.
Normal phase HPLC was used to measure retinoid levels. Rpe65(+/+), tvrm148/+ (T(+/-)), tvrm148/tvrm148 (T(-/-)), RPE65(KO/KO) (Rpe65(-/-)), and Rpe65(T/-) mice visual function was measured by optokinetic tracking (OKT) and electroretinography (ERG). Morphology was assessed by light microscopy and transmission electron microscopy (TEM). qRT-PCR was used to measure Rpe65 mRNA levels. Immunoblotting measured the size and amount of RPE65 protein.
The knockout and tvrm148 alleles did not complement. No 11-cis-retinal was detected in T(-/-) or Rpe65(-/-) mice. Visual acuity in Rpe65(+/+) and T(+/-) mouse was -0.382 c/d, but 0.037 c/d in T(-/-) mice at postnatal day 210 (P210). ERG response in T(-/-) mice was undetectable except at bright flash intensities. Outer nuclear layer (ONL) thickness in T(-/-) mice was -70% of Rpe65(+/+) by P210. Rpe65 mRNA levels in T(-/-) mice were unchanged, yet 14.5% of Rpe65(+/+) protein levels was detected. Protein size was unchanged.
A complementation test revealed the RPE65 knockout and tvrm148 alleles do not complement, proving that the tvrm148 mutation is in Rpe65. Behavioral, physiological, molecular, biochemical, and histological approaches indicate that tvrm148 is a null allele of Rpe65.
先前有报道称,一种名为 tvrm148 的小鼠突变可导致视网膜变性。Tvrm148 和 Rpe65 位于遗传图谱上的标记 D3Mit147 和 D3Mit19 之间,但物理图谱将 RPE65 置于标记之外。我们想知道是否是 Rpe65 或附近的其他基因发生了突变,以及突变是否降低了 11-顺式视黄醛水平。我们研究了 tvrm148 突变对视觉功能、形态和类视黄醇水平的影响。
采用正相高效液相色谱法测量类视黄醇水平。正常型 Rpe65(+/+)、tvrm148/+ (T(+/-))、tvrm148/tvrm148 (T(-/-))、RPE65(KO/KO) (Rpe65(-/-))和 Rpe65(T/-) 小鼠的视觉功能通过视动跟踪 (OKT) 和视网膜电图 (ERG) 进行测量。形态学通过光镜和透射电镜 (TEM) 评估。qRT-PCR 用于测量 Rpe65 mRNA 水平。免疫印迹用于测量 RPE65 蛋白的大小和含量。
敲除和 tvrm148 等位基因不能互补。在 T(-/-)或 Rpe65(-/-)小鼠中未检测到 11-顺式视黄醛。Rpe65(+/+)和 T(+/-)小鼠的视力为 -0.382 c/d,但 T(-/-)小鼠在出生后第 210 天 (P210) 时为 0.037 c/d。T(-/-)小鼠的 ERG 反应除在强闪光强度下外均无法检测到。T(-/-)小鼠的外核层 (ONL) 厚度在 P210 时为 Rpe65(+/+)的 -70%。T(-/-)小鼠的 Rpe65 mRNA 水平没有变化,但检测到 14.5%的 Rpe65(+/+)蛋白水平。蛋白大小不变。
互补测试表明,RPE65 敲除和 tvrm148 等位基因不能互补,证明 tvrm148 突变位于 Rpe65 上。行为、生理、分子、生化和组织学方法表明,tvrm148 是 Rpe65 的无效等位基因。