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<p><b>New page</b></p><div>[[File:Olympus_FluoView_FV1000_Confocal_Microscope_-_NCMIR.jpg|Olympus FluoView FV1000 Confocal Microscope - NCMIR|thumb]] '''Time-lapse microscopy''' is a powerful technique used in [[microscopy]] to observe and record the dynamic processes of living cells and tissues over time. This method involves capturing a series of images at specific intervals, which are then compiled into a video to visualize changes that occur over time.<br />
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==History==<br />
The development of time-lapse microscopy can be traced back to the early 20th century. It has evolved significantly with advancements in [[optical microscopy]], [[digital imaging]], and [[computer technology]]. Early pioneers in this field include [[Julius Ries]] and [[Jean Comandon]], who used time-lapse techniques to study cell division and microbial behavior.<br />
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==Principles==<br />
Time-lapse microscopy relies on the principles of [[optical microscopy]] and [[digital imaging]]. The basic setup includes a [[microscope]], a [[camera]], and a [[computer]] with specialized software. The camera captures images at predetermined intervals, and the software compiles these images into a time-lapse video.<br />
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==Applications==<br />
Time-lapse microscopy is widely used in various fields of [[biology]] and [[medicine]]. Some of the key applications include:<br />
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* [[Cell biology]]: Observing cell division, migration, and differentiation.<br />
* [[Developmental biology]]: Studying embryonic development and morphogenesis.<br />
* [[Neuroscience]]: Monitoring the growth and behavior of neurons.<br />
* [[Cancer research]]: Investigating tumor growth and metastasis.<br />
* [[Microbiology]]: Examining the behavior of microorganisms.<br />
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==Techniques==<br />
Several techniques are employed in time-lapse microscopy to enhance image quality and provide specific insights:<br />
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* [[Fluorescence microscopy]]: Uses fluorescent markers to highlight specific structures within cells.<br />
* [[Confocal microscopy]]: Provides high-resolution images by eliminating out-of-focus light.<br />
* [[Phase-contrast microscopy]]: Enhances contrast in transparent specimens without staining.<br />
* [[Differential interference contrast microscopy]]: Produces high-contrast images of unstained specimens.<br />
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==Advantages and Limitations==<br />
Time-lapse microscopy offers several advantages, including the ability to observe dynamic processes in real-time and the potential to capture rare or transient events. However, it also has limitations, such as phototoxicity, which can damage living cells, and the need for sophisticated equipment and software.<br />
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==Related Pages==<br />
* [[Microscopy]]<br />
* [[Fluorescence microscopy]]<br />
* [[Confocal microscopy]]<br />
* [[Cell biology]]<br />
* [[Developmental biology]]<br />
* [[Neuroscience]]<br />
* [[Cancer research]]<br />
* [[Microbiology]]<br />
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==References==<br />
{{Reflist}}<br />
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==External Links==<br />
{{Commons category|Time-lapse microscopy}}<br />
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[[Category:Microscopy]]<br />
[[Category:Cell biology]]<br />
[[Category:Biological techniques]]<br />
[[Category:Medical imaging]]<br />
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