Title :
Fluorescent microscope system to track a particular region of C. elegans
Author :
Maru, Mitsunori ; Igarashi, Yasunobu ; Arai, Shogo ; Hashimoto, Koichi
Author_Institution :
Dept. of Syst. Inf. Sci., Tohoku Univ., Sendai, Japan
Abstract :
C. elegans has been widely studied for understanding the basic mechanisms of nervous system function. In order to examine neural activity in C. elegans, it is necessary to measure a Ca2+ concentration in a neuron. Observers acquire fluorescence images of fluorescent dyes introduced in neurons. Then they can evaluate intensity of the fluorescence images which respond to changes in the Ca2+ concentration. Thus neural activity is examined by the fluorescence images of the neuron. However, observing the specified neuron in C. elegans for a long time is very difficult since a head of C. elegans moves quickly. To solve this problem, we develop a microscope system which can track a particular region of C. elegans and monitor fluorescence emitted by fluorescent protein in C. elegans. In experimental results, we show that the microscope system can track the head region of moving C. elegans and monitor fluorescence emitted by a chemosensory neuron ASER at 20× magnification.
Keywords :
biological techniques; cellular biophysics; chemioception; fluorescence spectroscopy; neurophysiology; optical microscopy; visible spectroscopy; zoology; ASER; C. elegans neural activity; C. elegans region tracking; Ca2+ concentration changes; Caenorhabditis elegans; chemosensory neuron; fluorescence image intensity; fluorescent dyes; fluorescent microscope system; nervous system function; neuron Ca2+ concentration; neuron fluorescence images; target tracking; Cameras; Head; Microscopy; Mirrors; Neurons; Optical filters; Proteins;
Conference_Titel :
System Integration (SII), 2010 IEEE/SICE International Symposium on
Conference_Location :
Sendai
Print_ISBN :
978-1-4244-9316-6
DOI :
10.1109/SII.2010.5708350
