![Figure 1. Pig CD47 does not interact with mouse SIRPα. (A) Western blot analysis of SIRPα tyrosine phosphorylation in WT mouse macrophages. Macrophages were incubated in medium alone (control; lane 1), or with CD47−/− mouse (lane 2), WT mouse (lane 3), or porcine (lane 4) RBCs for 30 minutes. (Rows 1-2) Macrophage lysates were used directly in Western blot with anti–β-actin (row 1, as a loading control) or with antiphosphotyrosine Ab (α-pTyr; row 2). (Row 3) Macrophage lysates were immunoprecipitated by anti-SIRPα mAb P84; precipitated proteins were then analyzed by Western blot with antiphosphotyrosine Ab (α-pTyr). A representative experiment of 3 is shown. (B) Blocking SIRPα by anti-SIRPα mAb (P84) augments phagocytosis of WT mouse, but not CD47−/− mouse or porcine RBCs. CFSE (green)–labeled splenic macrophages (5 × 105/well) were incubated with or without anti-SIRPα antibody (P84) in 96-well plate for 20 minutes; then PKH-26 (red)–stained WT mouse (WT), CD47 KO mouse (CD47−/−), untreated pig (pRBC), or opsonized pig (ops pRBC) RBCs (1 × 106/well) were added and phagocytosis was determined 1 hour after incubation using fluorescent microscope (engulfment was seen as a yellow event). The percent of macrophages engulfing target cells per well was calculated as follows: [number of yellow events/(number of yellow events + number of green nonengulfing macrophages)] × 100%. Data are presented as mean ± SDs (n = 10-12 wells per group). **P < .01.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/109/2/10.1182_blood-2006-04-019794/4/zh80020706720001.jpeg?Expires=1722795295&Signature=MAQNka6QU-6MwkCbdIy-vM-2~lhxCQpQsuFYm3QWbycfVoHbPfWp-31yykzI8Wr7JSUE1~ApTH6hNzT~yqqFWHKGF3btNXQeKEltJqSJsIqHFKOT9eQzO6brDX0D1PcgzhbYsCOl5C~kARRRpw0lWNz0iLyA95QXBBuksYRPaEeVthGDwKIrFORNYWRVcHrxmMDVvHqoISaOgo0MEXsqvM5ZH0XLCYdkHaM4otZ5oJl5~TxWyswrKg42FLoGHrWJA2fu9mePEc9lGqrbb1Mzm-17Pc3argPDb1bUqvWY7IsbdFO3yS8WXq7hOmnENOg~P8hgfG7gngWHcZ2YptxrCQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Pig CD47 does not interact with mouse SIRPα. (A) Western blot analysis of SIRPα tyrosine phosphorylation in WT mouse macrophages. Macrophages were incubated in medium alone (control; lane 1), or with CD47−/− mouse (lane 2), WT mouse (lane 3), or porcine (lane 4) RBCs for 30 minutes. (Rows 1-2) Macrophage lysates were used directly in Western blot with anti–β-actin (row 1, as a loading control) or with antiphosphotyrosine Ab (α-pTyr; row 2). (Row 3) Macrophage lysates were immunoprecipitated by anti-SIRPα mAb P84; precipitated proteins were then analyzed by Western blot with antiphosphotyrosine Ab (α-pTyr). A representative experiment of 3 is shown. (B) Blocking SIRPα by anti-SIRPα mAb (P84) augments phagocytosis of WT mouse, but not CD47−/− mouse or porcine RBCs. CFSE (green)–labeled splenic macrophages (5 × 105/well) were incubated with or without anti-SIRPα antibody (P84) in 96-well plate for 20 minutes; then PKH-26 (red)–stained WT mouse (WT), CD47 KO mouse (CD47−/−), untreated pig (pRBC), or opsonized pig (ops pRBC) RBCs (1 × 106/well) were added and phagocytosis was determined 1 hour after incubation using fluorescent microscope (engulfment was seen as a yellow event). The percent of macrophages engulfing target cells per well was calculated as follows: [number of yellow events/(number of yellow events + number of green nonengulfing macrophages)] × 100%. Data are presented as mean ± SDs (n = 10-12 wells per group). **P < .01.
