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Further, the C48A/C139A double mutant shows only monomeric behaviour.
In contrast with I323T, the TEA-insensitive Y294V (mSlo) mutant shows only one open level with a long open duration, indicating that its subunits have full cooperativity.
As discussed below, the CipA-ΔXDocII mutant shows only a small decrease in growth rate or cellulose degradation, and it is thus unlikely that the off-target insertion in this mutant has a substantial effect.
Despite shielding the active site in the apoenzyme and PAD·Ca(10mM 2+, R347 does not prevent calcium binding at Ca2 because the R347A mutant shows only a small effect on the concentration of calcium required for half maximal activity (i.e., K0.5; Table 1).
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In keeping with this notion, we found that the pri2(C4343A) mutant allele exhibited synthetic growth defect with sod1Δ; the double mutant is lethal at 30°C while each single mutant showed only mild growth defect (Fig. 7C).
Since the LinBUT I134V/A247H (=mutantmutant showed only weak LinBMI-type activity in our previous study (Ito et al. [2007]), cumulative mutations at the positions A112, I138, and M253 were introduced into the M2-1 mutant.
Interestingly, fadD1 mutant showed only increased swarming motility.
Mortality assays performed with the bscN mutant showed only a partial difference with K56-2 wild-type (Figure 5C).
In the latter species, even a ppsApckA double mutant showed only a marginal degree of attenuation indicating that gluconeogenesis plays, at most, a minor role for Salmonella virulence.
We found that the apc1 mutant showed only a 1.7-fold difference in centrosome and spindle misorientation (Figure 4C), indicating that the apc1 mutant is partially defective in the centrosome orientation checkpoint.
The pse1-1 kap123Δ mutant showed only a slight increase in cytoplasmic staining of GFP-eS26.
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