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GFP-Forked, a genetic reporter for studying <i>Drosophila</i> oocyte polarity
摘要: The polarized organization of the Drosophila oocyte can be visualized by examining the asymmetric localization of mRNAs, which is supported by networks of polarized microtubules (MTs). In this study, we used the gene forked, the putative Drosophila homologue of espin, to develop a unique genetic reporter for asymmetric oocyte organization. We generated a null allele of the forked gene using the CRISPR-Cas9 system and found that forked is not required for determining the axes of the Drosophila embryo. However, ectopic expression of a truncated form of GFP-Forked generated a distinct network of asymmetric Forked, which first accumulated at the oocyte posterior and was then restricted to the anterolateral region of the oocyte cortex in mid-oogenesis. This localization pattern resembled that reported for the polarized MTs network. Indeed, pharmacological and genetic manipulation of the polarized organization of the oocyte showed that the filamentous Forked network diffused throughout the entire cortical surface of the oocyte, as would be expected upon perturbation of oocyte polarization. Finally, we demonstrated that Forked associated with Short-stop and Patronin foci, which assemble non-centrosomal microtubule-organizing centers. Our results thus show that clear visualization of asymmetric GFP-Forked network localization can be used as a novel tool for studying oocyte polarity.
关键词: ncMTOC,Oocyte,Drosophila,Polarity,Forked,Microtubules,CRISPR
更新于2025-09-23 15:22:29
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Metabolic imaging with the use of?fluorescence lifetime imaging microscopy (FLIM) accurately detects mitochondrial dysfunction in?mouse oocytes
摘要: To determine whether metabolic imaging with the use of fluorescence lifetime imaging microscopy (FLIM) identifies metabolic differences between normal oocytes and those with metabolic dysfunction. Experimental study. Academic research laboratories. None. Oocytes from mice with global knockout of Clpp (caseinolytic peptidase P; n ? 52) were compared with wild-type (WT) oocytes (n ? 55) as a model of severe oocyte dysfunction. Oocytes from old mice (1 year old; n ? 29) were compared with oocytes from young mice (12 weeks old; n ? 35) as a model of mild oocyte dysfunction. FLIM was used to measure the naturally occurring nicotinamide adenine dinucleotide dehydrogenase (NADH) and flavin adenine dinucleotide (FAD) autofluorescence in individual oocytes. Eight metabolic parameters were obtained from each measurement (4 per fluorophore): short (t1) and long (t2) fluorescence lifetime, fluorescence intensity (I), and fraction of the molecule engaged with enzyme (F). Reactive oxygen species (ROS) levels and blastocyst development rates were measured to assess illumination safety. In Clpp-knockout oocytes compared with WT, FAD t1 and t2 were longer and I was higher, NADH t2 was longer, and F was lower. In old oocytes compared with young ones, FAD t1 was longer and I was lower, NADH t1 and t2 were shorter, and I and F were lower. FLIM did not affect ROS levels or blastocyst development rates. FLIM parameters exhibit strong differentiation between Clpp-knockout versus WT, and old versus young oocytes. FLIM could potentially be used as a noninvasive tool to assess mitochondrial function in oocytes.
关键词: Mitochondria,aging,mitochondrial unfolded protein response,fluorescence lifetime imaging microscopy,CLPP,FLIM,oocyte
更新于2025-09-10 09:29:36