Thank you very much for developing MiloR. I have a question regarding the analysis process. In MiloR, KNN neighborhoods are constructed first, and then the number of cells present in each neighborhood is counted (for each experimental sample) and used for differential abundance testing between conditions.
However, if some technical issue causes a certain cell population (e.g., plasma cells) to be particularly abundant in one sample (sample X) while being nearly absent in all other samples, and this sample X happens to belong to the treatment group, then in the MiloR analysis plasma cells would likely appear to be more abundant in the treatment group. Yet such a result would not be biological. I would like to ask whether MiloR has any correction approach to handle this kind of situation.
Thank you very much for developing MiloR. I have a question regarding the analysis process. In MiloR, KNN neighborhoods are constructed first, and then the number of cells present in each neighborhood is counted (for each experimental sample) and used for differential abundance testing between conditions.
However, if some technical issue causes a certain cell population (e.g., plasma cells) to be particularly abundant in one sample (sample X) while being nearly absent in all other samples, and this sample X happens to belong to the treatment group, then in the MiloR analysis plasma cells would likely appear to be more abundant in the treatment group. Yet such a result would not be biological. I would like to ask whether MiloR has any correction approach to handle this kind of situation.