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A rapid population method for action spectra applied to Halobacterium halobium.

机译:一种适用于卤化嗜盐杆菌的作用谱快速填充方法。

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摘要

We have developed a simple and rapid technique for measuring the action spectra for phototaxis of populations of microorganisms and applied it to halobacteria. A microscope with a dark-field condenser was used to illuminate the cell suspension in a sealed chamber with light of wavelength greater than 750 nm; in this region of the spectrum, the halobacteria show no phototactic response. A 150-micron spot of light from a xenon arc lamp, whose wavelength and intensity can be varied, was projected through the objective lens into the center of the dark field. The objective lens imaged this measuring spot through a 780-nm cut-off filter on an aperture in front of a photomultiplier. The intensity of the scattered 750-nm light, and therefore the photomultiplier current, is proportional to the number of cells in the measuring spot. A third lamp provided background light of variable wavelength and intensity through the dark-field condenser. To minimize secondary effects due to large changes in cell density, we recorded the initial changes in the photomultiplier current over 1 min after the actinic light had been switched on. By plotting the rate of change against wavelength, we obtained action spectra after the proper corrections for changes in light intensity with wavelength were applied and saturation effects were avoided.
机译:我们已经开发出一种简单而快速的技术来测量微生物群体趋光性的作用谱,并将其应用于盐菌。使用带有暗场聚光镜的显微镜以波长大于750 nm的光照射密封室中的细胞悬液。在该光谱区域中,盐杆菌没有显示出光战术反应。氙弧灯发出的150微米光点(其波长和强度可以改变)通过物镜投射到暗场的中心。物镜通过一个光电倍增管前面的孔径上的780 nm截止滤光片对该测量点成像。 750 nm散射光的强度以及光电倍增管电流与测量点中的细胞数量成正比。第三盏灯通过暗场聚光镜提供波长和强度可变的背景光。为了最大程度地减少由于细胞密度的大变化而引起的二次效应,我们在接通光化光后的1分钟内记录了光电倍增管电流的初始变化。通过绘制变化率与波长的关系图,在对光强度随波长的变化进行了适当的校正并避免了饱和效应之后,我们获得了作用谱。

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