Intercalated cells are known to be involved in acid-base homeostasis via vacuolar ATPase (H+-ATPase or V-ATPase) expression. Increasing evidence supports an innate immune role for ICs along with their traditional function of pH regulation. In this study, human kidney tissue was enriched for viable intercalated cells then exposed to uropathogenic E. coli versus saline control. Single cell transcriptomics was performed. Six intercalated cell subtypes were identified including hybrid principal-intercalated cells. Cell specific cluster marker gene list generated from this sequencing data was put through ingenuity pathway analysis pipeline which predicted “phagosome maturation” as a key biological pathway that increased in rank following exposure to uropathogenic E. coli in two of the intercalated cell subtypes. Uptake of E. coli and pHrodo coated E. coli BioParticlesTM during live animal intravital microscopy demonstrated that intercalated cell phagocytosis of bacteria was an active process that involved acidification. Taken together, our finding indicate that intercalated cells represent an epithelial cell with characteristics of professional phagocytes like macrophages or neutrophils, which includes the ability to phagocytose E. coli and acidify phagolysosomes. Overall design: Normal margin of the human kidney biopsy sample was processed for single cell suspension with enzymatic digestion (Liberase TL and DNAse I) and rapid dissociation using GentleMacs (Miltenyi Biotec). Dead cells were then removed from single cell suspension using dead cell removal microbead (Miltenyi Biotec). CD45+ traditional immune cells were then removed using anti-human CD45 microeads (Miltenyi Biotec). Intercalated cells were then enriched using anti-human C-KIT (CD117) microbeads (Miltenyi Biotec). Cell viability was tested on hemocytometer. Viable cells were equally divided into 2 wells of the 96-well U bottom plate and exposed to uropathogenic E.coli (UPEC) for 1 hr and sterile saline at 370C and 5% CO2 environment. After washing with sterile PBS and re-suspension in PBS (without Ca2+ and Mg2+) both cells samples (Saline control and UPEC exposed) were immediately processed for single cell sequencing using 10x genomics platform. Single cells of both samples were sequenced on Illumina Novaseq 6000 instrument.