![Circulating MKs are increased in COVID-19. (A) scRNA-seq dimensionality reduction using uniform manifold approximation and projection of 317 562 cells derived from 4 separate studies. MKs (4180 cells) are shown in red. (B) scRNA-seq marker genes used to identify circulating MKs. (C) Frequency of MKs relative to all cells from scRNA-seq samples. Median ± minimum/maximum. Kruskal–Wallis one-way ANOVA with Dunn post hoc multiple comparisons test. All groups compared with uninfected control. Adjusted P value ∗∗∗P = .001 to .0001. Mild-moderate: n = 15; severe: n = 14; early recovery (<7 days after first negative polymerase chain reaction [PCR] test): n = 8; late recovery (>14 days after first negative PCR test): n = 8; uninfected: n = 19. (D) Flow cytometry from UAB COVID-19 peripheral blood samples (n = 20) showing gating of CD61+ CD41+ DNA–positive MKs. The histogram shows ploidy distribution ranging from 2n to 32n. (E) Cytocentrifugation of FACS-sorted MKs stained with hematoxylin and eosin. (F) Representative flow cytometry plots showing the proportion of MKs relative to platelets in uninfected vs COVID-19 peripheral blood. (G) Quantification of MK frequency, relative to all live events, using flow cytometry on peripheral blood from uninfected (n = 9 donors) vs COVID-19 (n = 218 patients; 220 samples). Mean ± standard error of the mean (SEM). Unpaired 2-tailed t test with Welch correction; ∗∗∗∗P < .0001. ANOVA, analysis of variance.](https://ash.silverchair-cdn.com/ash/content_public/journal/bloodadvances/7/15/10.1182_bloodadvances.2022009022/1/blooda_adv-2022-009022-gr1.jpeg?Expires=1724949643&Signature=LCxnIiV0oaCKdiBE4a~dEcvJ8VcYQgf81K4IsPmAmGhGAHBcRopN3DOlTNF-XhQZJROmPwYCgqS424wakhEhO0oGeOy0~gDw6NZ3XTFejXyqhCHnQBtksx0YrUe-BnXaUKFViP6oRVFjyEkDLoqVfbJD1vVBmm8wzWgKC4CrxA7bkFIXwAlQgRw69zZVLXE2AvKoHoxYexmPxK25s3OVDM2Bt3juechQyCWuIwZHTQJ1BalT4hUNc5l6aM51nicqlYBelDoq8uRfh9R~TyloPNOwrQ8TeOk3RYBjh3w-hey7eISt3HN5JFMrwlzTYVMVwingu97WwbQflE1rmg29vQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Circulating MKs are increased in COVID-19. (A) scRNA-seq dimensionality reduction using uniform manifold approximation and projection of 317 562 cells derived from 4 separate studies. MKs (4180 cells) are shown in red. (B) scRNA-seq marker genes used to identify circulating MKs. (C) Frequency of MKs relative to all cells from scRNA-seq samples. Median ± minimum/maximum. Kruskal–Wallis one-way ANOVA with Dunn post hoc multiple comparisons test. All groups compared with uninfected control. Adjusted P value ∗∗∗P = .001 to .0001. Mild-moderate: n = 15; severe: n = 14; early recovery (<7 days after first negative polymerase chain reaction [PCR] test): n = 8; late recovery (>14 days after first negative PCR test): n = 8; uninfected: n = 19. (D) Flow cytometry from UAB COVID-19 peripheral blood samples (n = 20) showing gating of CD61+ CD41+ DNA–positive MKs. The histogram shows ploidy distribution ranging from 2n to 32n. (E) Cytocentrifugation of FACS-sorted MKs stained with hematoxylin and eosin. (F) Representative flow cytometry plots showing the proportion of MKs relative to platelets in uninfected vs COVID-19 peripheral blood. (G) Quantification of MK frequency, relative to all live events, using flow cytometry on peripheral blood from uninfected (n = 9 donors) vs COVID-19 (n = 218 patients; 220 samples). Mean ± standard error of the mean (SEM). Unpaired 2-tailed t test with Welch correction; ∗∗∗∗P < .0001. ANOVA, analysis of variance.
