Automated quantification of photoreceptor outer segments in developing and degenerating retinas on microscopy images across scales

IF 3.5 3区医学 Q2 NEUROSCIENCES

Frontiers in Molecular Neuroscience Pub Date : 2024-05-24 DOI:10.3389/fnmol.2024.1398447

Suse Seidemann, Florian Salomon, K. Hoffmann, Thomas Kurth, Ivo F. Sbalzarini, Robert Haase, Marius Ader

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引用次数: 0

Abstract

The functionality of photoreceptors, rods, and cones is highly dependent on their outer segments (POS), a cellular compartment containing highly organized membranous structures that generate biochemical signals from incident light. While POS formation and degeneration are qualitatively assessed on microscopy images, reliable methodology for quantitative analyses is still limited. Here, we developed methods to quantify POS (QuaPOS) maturation and quality on retinal sections using automated image analyses. POS formation was examined during the development and in adulthood of wild-type mice via light microscopy (LM) and transmission electron microscopy (TEM). To quantify the number, size, shape, and fluorescence intensity of POS, retinal cryosections were immunostained for the cone POS marker S-opsin. Fluorescence images were used to train the robust classifier QuaPOS-LM based on supervised machine learning for automated image segmentation. Characteristic features of segmentation results were extracted to quantify the maturation of cone POS. Subsequently, this quantification method was applied to characterize POS degeneration in “cone photoreceptor function loss 1” mice. TEM images were used to establish the ultrastructural quantification method QuaPOS-TEM for the alignment of POS membranes. Images were analyzed using a custom-written MATLAB code to extract the orientation of membranes from the image gradient and their alignment (coherency). This analysis was used to quantify the POS morphology of wild-type and two inherited retinal degeneration (“retinal degeneration 19” and “rhodopsin knock-out”) mouse lines. Both automated analysis technologies provided robust characterization and quantification of POS based on LM or TEM images. Automated image segmentation by the classifier QuaPOS-LM and analysis of the orientation of membrane stacks by QuaPOS-TEM using fluorescent or TEM images allowed quantitative evaluation of POS formation and quality. The assessments showed an increase in POS number, volume, and membrane coherency during wild-type postnatal development, while a decrease in all three observables was detected in different retinal degeneration mouse models. All the code used for the presented analysis is open source, including example datasets to reproduce the findings. Hence, the QuaPOS quantification methods are useful for in-depth characterization of POS on retinal sections in developmental studies, for disease modeling, or after therapeutic interventions affecting photoreceptors.

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在不同尺度的显微镜图像上自动量化发育中和退化中视网膜的感光体外节段

光感受器、视杆细胞和视锥细胞的功能高度依赖于它们的外节（POS），这是一个包含高度组织化的膜结构的细胞区，能从入射光中产生生化信号。虽然可以通过显微镜图像对 POS 的形成和退化进行定性评估，但用于定量分析的可靠方法仍然有限。在此，我们开发了利用自动图像分析方法来量化视网膜切片上的 POS（QuaPOS）成熟度和质量。我们通过光学显微镜（LM）和透射电子显微镜（TEM）对野生型小鼠在发育期和成年期的 POS 形成进行了检测。为了量化POS的数量、大小、形状和荧光强度，对视网膜冷冻切片进行了锥体POS标记物S-眼球蛋白的免疫染色。荧光图像用于训练基于监督机器学习的鲁棒分类器 QuaPOS-LM，以实现自动图像分割。提取分割结果的特征来量化锥体 POS 的成熟度。随后，这种量化方法被用于描述 "视锥感光器功能缺失 1 "小鼠的 POS 退化特征。利用 TEM 图像建立了用于 POS 膜排列的超微结构量化方法 QuaPOS-TEM。使用定制的 MATLAB 代码分析图像，从图像梯度中提取膜的方向及其排列（一致性）。这种分析方法被用于量化野生型小鼠和两种遗传性视网膜变性（"视网膜变性 19 "和 "视紫红质基因敲除"）小鼠品系的 POS 形态。这两种自动分析技术都能根据 LM 或 TEM 图像对 POS 进行可靠的表征和量化。利用荧光图像或 TEM 图像，QuaPOS-LM 分类器可自动分割图像，QuaPOS-TEM 可分析膜堆的方向，从而对 POS 的形成和质量进行定量评估。评估结果表明，在野生型小鼠出生后的发育过程中，POS的数量、体积和膜的连贯性都有所增加，而在不同的视网膜变性小鼠模型中，这三个观察指标都有所下降。本文分析所用的所有代码都是开源的，包括用于重现研究结果的示例数据集。因此，QuaPOS 定量方法有助于在发育研究、疾病建模或影响光感受器的治疗干预后深入表征视网膜切片上的 POS。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Frontiers in Molecular Neuroscience NEUROSCIENCES-

CiteScore

5.70

自引率

2.10%

发文量

669

审稿时长

14 weeks

期刊介绍： Frontiers in Molecular Neuroscience is a first-tier electronic journal devoted to identifying key molecules, as well as their functions and interactions, that underlie the structure, design and function of the brain across all levels. The scope of our journal encompasses synaptic and cellular proteins, coding and non-coding RNA, and molecular mechanisms regulating cellular and dendritic RNA translation. In recent years, a plethora of new cellular and synaptic players have been identified from reduced systems, such as neuronal cultures, but the relevance of these molecules in terms of cellular and synaptic function and plasticity in the living brain and its circuits has not been validated. The effects of spine growth and density observed using gene products identified from in vitro work are frequently not reproduced in vivo. Our journal is particularly interested in studies on genetically engineered model organisms (C. elegans, Drosophila, mouse), in which alterations in key molecules underlying cellular and synaptic function and plasticity produce defined anatomical, physiological and behavioral changes. In the mouse, genetic alterations limited to particular neural circuits (olfactory bulb, motor cortex, cortical layers, hippocampal subfields, cerebellum), preferably regulated in time and on demand, are of special interest, as they sidestep potential compensatory developmental effects.