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1. Testing the LSST Difference Image Analysis Pipeline Using Synthetic Source Injection Analysis

   https://doi.org/10.3847/1538-4357/ad3635  

   Liu, S; Wood-Vasey, W M; Armstrong, R; Narayan, G; Sánchez, B O (May 2024, The Astrophysical Journal)

   Abstract We evaluate the performance of the Legacy Survey of Space and Time Science Pipelines Difference Image Analysis (DIA) on simulated images. By adding synthetic sources to galaxies on images, we trace the recovery of injected synthetic sources to evaluate the pipeline on images from the Dark Energy Science Collaboration Data Challenge 2. The pipeline performs well, with efficiency and flux accuracy consistent with the signal-to-noise ratio of the input images. We explore different spatial degrees of freedom for the Alard–Lupton polynomial-Gaussian image subtraction kernel and analyze for trade-offs in efficiency versus artifact rate. Increasing the kernel spatial degrees of freedom reduces the artifact rate without loss of efficiency. The flux measurements with different kernel spatial degrees of freedom are consistent. We also here provide a set of DIA flags that substantially filter out artifacts from the DIA source table. We explore the morphology and possible origins of the observed remaining subtraction artifacts and suggest that given the complexity of these artifact origins, a convolution kernel with a set of flexible bases with spatial variation may be needed to yield further improvements. 

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2. F-BAR Cdc15 Promotes Cdc42 Activation During Cytokinesis and Cell Polarization in Schizosaccharomyces pombe

   https://doi.org/10.1534/genetics.119.302649  

   Hercyk, Brian S; Das, Maitreyi E (December 2019, Genetics)

   Abstract Cdc42, a Rho-family GTPase, is a master regulator of cell polarity. Recently, it has been shown that Cdc42 also facilitates proper cytokinesis in the fission yeast Schizosaccharomyces pombe. Cdc42 is activated by two partially redundant GEFs, Gef1 and Scd1. Although both GEFs activate Cdc42, their deletion mutants display distinct phenotypes, indicating that they are differentially regulated by an unknown mechanism. During cytokinesis, Gef1 localizes to the division site and activates Cdc42 to initiate ring constriction and septum ingression. Here, we report that the F-BAR protein Cdc15 promotes Gef1 localization to its functional sites. We show that cdc15 promotes Gef1 association with cortical puncta at the incipient division site to activate Cdc42 during ring assembly. Moreover, cdc15 phospho-mutants phenocopy the polarity phenotypes of gef1 mutants. In a hypermorphic cdc15 mutant, Gef1 localizes precociously to the division site and is readily detected at the cortical patches and the cell cortex. Correspondingly, the hypermorphic cdc15 mutant shows increased bipolarity during interphase and precocious Cdc42 activation at the division site during cytokinesis. Finally, loss of gef1 in hypermorphic cdc15 mutants abrogates the increased bipolarity and precocious Cdc42 activation phenotype. We did not see any change in the localization of the other GEF Scd1 in a Cdc15-dependent manner. Our data indicate that Cdc15 facilitates Cdc42 activation at the division site during cytokinesis at the cell cortex to promote bipolarity and this is mediated by promoting Gef1 localization to these sites. 

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3. Endocytic patch dynamics are differentially regulated at distinct cell sites in fission yeast

   https://doi.org/10.1242/jcs.263873  

   Campbell, Bethany_F; Kalathil, Dhanya; Patel, Uma_J; Williams, Ashlei_R; Das, Maitreyi_E (August 2025, Journal of Cell Science)

   Endocytosis promotes polarity and growth in eukaryotes. In Schizosaccharomyces pombe fission yeast, endocytosis occurs at the polarized cell ends and division site and at the non-polarized cell sides. Our characterization of endocytic actin patches show that they are differentially regulated. The patches at the cell ends and division site internalize successfully while those at the sides are weak and erratic. The major regulator of cell polarity, Cdc42, and its target Pak1 kinase only localize to the cell ends and division site. We find that these proteins regulate assembly and internalization of patches at these sites but not at the cell sides. Moreover, Cdc42 specifically activated by the GEF Gef1 promotes proper patch dynamics. Endocytosis requires phosphorylation of the Type I Myosin Myo1 by the Pak1 kinase. Myo1 localizes to the cell ends, division site, and the cell sides. We find that unlike Cdc42 and Pak1, Myo1 also promotes patch assembly at the cell sides. Our data indicate that while Myo1 can globally promote branched actin assembly, successful endocytic patch dynamics and internalization at polarized sites require Cdc42 and Pak1 kinase. 

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4. A suppressor tRNA-mediated feedforward loop eliminates leaky gene expression in bacteria

   https://doi.org/10.1093/nar/gkaa1179  

   Ho, Joanne M; Miller, Corwin A; Parks, Sydney E; Mattia, Jacob R; Bennett, Matthew R (December 2020, Nucleic Acids Research)

   null (Ed.)

   Abstract Ligand-inducible genetic systems are the mainstay of synthetic biology, allowing gene expression to be controlled by the presence of a small molecule. However, ‘leaky’ gene expression in the absence of inducer remains a persistent problem. We developed a leak dampener tool that drastically reduces the leak of inducible genetic systems while retaining signal in Escherichia coli. Our system relies on a coherent feedforward loop featuring a suppressor tRNA that enables conditional readthrough of silent non-sense mutations in a regulated gene, and this approach can be applied to any ligand-inducible transcription factor. We demonstrate proof-of-principle of our system with the lactate biosensor LldR and the arabinose biosensor AraC, which displayed a 70-fold and 630-fold change in output after induction of a fluorescence reporter, respectively, without any background subtraction. Application of the tool to an arabinose-inducible mutagenesis plasmid led to a 540-fold change in its output after induction, with leak decreasing to the level of background mutagenesis. This study provides a modular tool for reducing leak and improving the fold-induction within genetic circuits, demonstrated here using two types of biosensors relevant to cancer detection and genetic engineering. 

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5. Measuring the spectral response of a division-of-focal-plane polarization imager using a grating monochromator

   https://doi.org/10.1364/AO.454801  

   Venkatesulu, Erica; Shaw, Joseph_A (March 2022, Applied Optics)

   Spectral characterizations are performed on imagers to obtain a relative spectral response (RSR) curve. This process often utilizes a grating monochromator with an output that changes polarization as a function of wavelength (our monochromator’s degree of linear polarization was found to vary from less than 10% to more than 70%). When characterizing a polarization-sensitive imager, this introduces polarization artifacts into the RSR curve. We present a simple method to avoid these polarization artifacts for division-of-focal-plane polarization imagers by directly illuminating the camera with the monochromator output and calculating the S₀Stokes parameter at each super pixel, then we show consistent results from this method for two division-of-focal-plane polarization imagers. We also show that ignoring the monochromator polarization results in order-of-magnitude RSR errors. The recommended method uses an iris to limit the spatial extent of the monochromator output, which was found experimentally to increase the minimum signal-to-noise ratio by more than a factor of 2. 

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