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一种定量分析黄斑和视乳头周围血管光学相干断层扫描血管造影图像的标准化方法。

A standardized method to quantitatively analyze optical coherence tomography angiography images of the macular and peripapillary vessels.

作者信息

Mello Luiz Guilherme Marchesi, Rodrigues Neto Taurino Dos Santos, da Silva Neto Epitácio Dias, Preti Rony Carlos, Monteiro Mário Luiz Ribeiro, Zacharias Leandro Cabral

机构信息

Department of Specialized Medicine, Centro de Ciências da Saúde (CCS), Universidade Federal do Espírito Santo, Vitória, Brazil.

Division of Ophthalmology and the Laboratory for Investigation in Ophthalmology (LIM-33), Faculdade de Medicina FMUSP, Universidade de São Paulo, Av. Dr Enéas de Carvalho Aguiar, 255, Cerqueira César, São Paulo, 05403-001, Brazil.

出版信息

Int J Retina Vitreous. 2022 Oct 15;8(1):75. doi: 10.1186/s40942-022-00426-9.

Abstract

BACKGROUND

Optical coherence tomography angiography (OCTA) is a relatively new non-invasive imaging technique to evaluate retinal vascular complexes. However, there is still a lack of standardization and reproducibility of its quantitative evaluation. Furthermore, manual analysis of a large amount of OCTA images makes the process laborious, with greater data variability, and risk of bias. Therefore, the aim of this study is to describe a fast and reproducible quantitative analysis of the foveal avascular zone (FAZ), macular superficial and deep vascular complexes (mSVC and mDVC, respectively), and peripapillary superficial vascular complex (pSVC) in OCTA images.

METHODS

We survey models and methods used for studying retinal microvasculature, and software packages used to quantify microvascular networks. These programs have provided researchers with invaluable tools, but we estimate that they have collectively achieved low adoption rates, possibly due to complexity for unfamiliar researchers and nonstandard sets of quantification metrics. To address these existing limitations, we discuss opportunities to improve effectiveness, affordability, and reproducibility of microvascular network quantification with the development of an automated method to analyze the vessels and better serve the current and future needs of microvascular research. OCTA images of the macula (10°x10°, 15°x15°, or 20°x20° centered on the fovea) and peripapillary area (15 × 15º centered on optic nerve head) were exported from the device and processed using the open-source software Fiji. The mSVC, mDVC, and pSVC were automatically analyzed regarding vascular density in the total area and four sectors (superior, inferior, nasal, and temporal). We also analyzed the FAZ regarding its area, perimeter, and circularity in the SVC and DVC images.

RESULTS

We developed an automated model and discussed a step by step method to analyze vessel density and FAZ of the macular SVC and DVC, acquired with OCTA using different fields of view. We also developed an automated analysis of the peripapillary SVC.

CONCLUSION

Our developed automated analysis of macular and peripapillary OCTA images will allow a fast, reproducible, and precise quantification of SVC, DVC, and FAZ. It would also allow more accurate comparisons between different studies and streamlines the processing of images from multiple patients with a single command.

摘要

背景

光学相干断层扫描血管造影(OCTA)是一种相对较新的用于评估视网膜血管复合体的非侵入性成像技术。然而,其定量评估仍缺乏标准化和可重复性。此外,对大量OCTA图像进行手动分析会使过程繁琐,数据变异性更大,且存在偏差风险。因此,本研究的目的是描述一种对OCTA图像中黄斑无血管区(FAZ)、黄斑浅层和深层血管复合体(分别为mSVC和mDVC)以及视乳头周围浅层血管复合体(pSVC)进行快速且可重复的定量分析方法。

方法

我们调研了用于研究视网膜微血管的模型和方法,以及用于量化微血管网络的软件包。这些程序为研究人员提供了宝贵的工具,但我们估计它们的总体采用率较低,这可能是由于对于不熟悉的研究人员来说较为复杂,以及量化指标集不标准。为了解决这些现有局限性,我们讨论了随着一种自动分析血管的方法的发展,提高微血管网络量化的有效性、可承受性和可重复性的机会,以更好地满足当前和未来微血管研究的需求。从设备中导出黄斑(以黄斑为中心的10°×10°、15°×15°或20°×20°)和视乳头周围区域(以视乳头为中心的15×15º)的OCTA图像,并使用开源软件Fiji进行处理。对mSVC、mDVC和pSVC在总面积和四个扇区(上、下、鼻侧和颞侧)的血管密度进行自动分析。我们还在SVC和DVC图像中分析了FAZ的面积、周长和圆形度。

结果

我们开发了一种自动模型,并讨论了一种逐步分析使用不同视野的OCTA获取的黄斑SVC和DVC的血管密度和FAZ的方法。我们还开发了对视乳头周围SVC进行自动分析的方法。

结论

我们开发的对黄斑和视乳头周围OCTA图像的自动分析将允许对SVC、DVC和FAZ进行快速、可重复且精确的量化。它还将允许在不同研究之间进行更准确的比较,并通过单个命令简化对多名患者图像的处理。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7a87/9569066/586e145c9fb0/40942_2022_426_Fig1_HTML.jpg

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