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Non-transfected PC12 cells (NT) and cells transfected with either wild type human ZnT3-myc or ZnT3 tyrosine mutants were stained with zinquin (Fig. 5C).
Controls and mutants were stained simultaneously using the same solutions, in the same Eppendorf tubes or glass vials, and imaged on the same days using identical microscope settings.
To measure mitochondrial superoxides, cells overexpressing Magmas and Magmas mutants were stained with 25 μM MitoSOX for 15 min and mounted in ProLong Gold Antifade reagent with DAPI (Invitrogen).
Very similar images of stretched kinetochores were also observed when the mutants were stained for tagged versions of various other kinetochore proteins such as CENP-CCnp3, Mis12, Nuf2, and Sim4 (data not shown, and below).
The wild type, fat-5, fat-6 and fat-7 mutants, as well as fat-5 fat-6 and fat-5 fat-6 double mutands were stained with both the vital dye Nile Red and with the fat-5 fat-7e Oil Red-O, both ofat-5 fat-7e previously been usedoubleharacterize fat storage in C. elegans [ 12, 21].
DOI: http://dx.doi.org/10.7554/eLife.07074.010 To confirm that the phenotypic basis of the selective advantage is similar to the previously described WS mutants (where activation of a DGC results in overproduction of cellulose [ McDonald et al., 2009]) reconstructed mutants were stained with calcofluor and Congo red and their colony morphology examined.
Similar(54)
Next, a series of Δ Afchs disruption mutants was stained with CFW to establish which CHS enzymes were required for the compensatory increase in chitin synthesis induced by exposure to caspofungin (Fig. 4i).
The kidney tissue sections from transgenic founders, chimeric mice with wild type HNF-1β and HNF-1β deletion mutant, were stained with collectrin antibody (red) and V5 antibody (green) (Figure 1d) and nuclei were counterstained blue with 4'-6-diamidino-2-phenylindole.
The pollen grains in the WT and the mutant were stained with 2% I2-KI to detect starch activity during the flowering period.
Pollen grains in the WT and GMS mutant were stained with 2% I2-KI to detect starch activity at 0 DPA.
Approximately 4% of small buds of the chs2Δ chs8Δ mutant were stained with PI indicating that death occurred during early polarized growth in these cells (Fig. 1A,B and Table 2).
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Justyna Jupowicz-Kozak
CEO of Professional Science Editing for Scientists @ prosciediting.com