![MKL1-deficient neutrophils are defective in actin polymerization and have reduced actin levels. Actin polymerization was examined in suspension after stimulation with fMLF (10 nM) or C5a (10 nM) (mean ± range, n = 2 of the index patient) (A) and by confocal analysis with staining for F-actin (magenta = F-actin [phalloidin], cyan = DNA [Hoechst]) upon a 10-minute stimulation with fMLF (B). Images were acquired with a Leica TCS SP8 confocal microscope. Scale bars, 10 µm. (C) Cytospins of isolated neutrophils from control and index patient samples (original magnification ×400; May-Grünwald-Giemsa stain). (D) Reduced actin levels in MKL1-deficient neutrophils were detected using western blotting with anti-actin. GAPDH was used as loading control (n = 2 of the index case). (E) Quantification of actin levels in panel D. (F) Representative immuno-electron microscopy images stained for anti-actin (black dots). The pseudopodia were more bluntly shaped compared with control neutrophils (lower panels). Images were acquired with a Tecnai 12 G2 transmission electron microscope. Scale bars, 1 µm. (G) Quantification of gold-labeled particles in immuno-electron microscopy images stained for anti-actin (n = 1 of the index patient and control; 4 images were analyzed per donor). C, control; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; P, patient.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/135/24/10.1182_blood.2019002633/3/bloodbld2019002633f2.png?Expires=1724876012&Signature=jbmx67TBUASTsW6mDEXdHIvitMw95k4joqOLlbE8nWGrrEt5LgTEO7-w9KyHSqCbNQOjx4WgbxDnMtLt5H1ECwjqQZvCQGQFo7uVtw7tAMh8XvtfRAi2pqf-OdLn~pgijoPGhn6YMd6Cw4NQkWOPsboU4mMPYbDYbzfGDQpayvOKG-oIIpzry20h3EIe3L6ma5HrlK7N11tc5Ml7E3vJ3x65cR6Ym3bhUYoOce-ND97l~Ic4SYVyF5PvMM00nISl8KIexRQ9xJdpstzhTVgdDtcDd36QFL~cX7ukTgTCTlr-siMHInwvN7sB2w2ANFHghU89ODAjs3vOAvY1plW4NA__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
MKL1-deficient neutrophils are defective in actin polymerization and have reduced actin levels. Actin polymerization was examined in suspension after stimulation with fMLF (10 nM) or C5a (10 nM) (mean ± range, n = 2 of the index patient) (A) and by confocal analysis with staining for F-actin (magenta = F-actin [phalloidin], cyan = DNA [Hoechst]) upon a 10-minute stimulation with fMLF (B). Images were acquired with a Leica TCS SP8 confocal microscope. Scale bars, 10 µm. (C) Cytospins of isolated neutrophils from control and index patient samples (original magnification ×400; May-Grünwald-Giemsa stain). (D) Reduced actin levels in MKL1-deficient neutrophils were detected using western blotting with anti-actin. GAPDH was used as loading control (n = 2 of the index case). (E) Quantification of actin levels in panel D. (F) Representative immuno-electron microscopy images stained for anti-actin (black dots). The pseudopodia were more bluntly shaped compared with control neutrophils (lower panels). Images were acquired with a Tecnai 12 G2 transmission electron microscope. Scale bars, 1 µm. (G) Quantification of gold-labeled particles in immuno-electron microscopy images stained for anti-actin (n = 1 of the index patient and control; 4 images were analyzed per donor). C, control; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; P, patient.