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To determine the effect of 8-oxodG bypass in the presence of all four human Y-family DNA polymerases in vitro, a running start assay was performed with an equal molar concentration of all four human Y-family enzymes.
Nevertheless, the running start assay indicated that the 8-oxodG lesion reduced the activity of this polymerase as hRev1 extended the control DNA substrate to a 23-mer but was only capable of extending the damaged DNA substrate to a 21-mer product.
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Genetic studies in non-model organisms will be facilitated greatly - with these methods it is now possible to start assaying genetic variability across many samples without the time and expense of building a reference genome.
Running start assays performed with the combination of hPolη, hPolκ, and hPolι lack this 18-mer product, indicating that the accumulation of the 18-mer product in the presence of all four enzymes is indeed due to hRev1.
Analysis of the running start assays was performed as previously described by calculating the relative lesion bypass efficiencies (8-oxodG bypass%) of each polymerase as a function of reaction time.
In contrast, in running start assays with Dpo4 where a stretch of a template is replicated in the presence of all four dNTPs starting several positions upstream from a DNA lesion, a significant accumulation of intermediate products corresponding to incorporations opposite and adjacent to the lesion has been observed for a number of DNA lesions.
Prepare all standards before starting assay procedure.
Of 4 patients, not enough cells were retrieved to start the assay.
The cells were warmed to 35°C to start the assay.
The PM consists of two components, which are combined to start the assay.
Silique total soluble protein was added 30 min after the start of assay.
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