Multiphoton In Vivo Microscopy of Embryonic Thrombopoiesis Reveals the Generation of Platelets through Budding

Author:

Liu Huan1,Ishikawa-Ankerhold Hellen1ORCID,Winterhalter Julia1,Lorenz Michael1,Vladymyrov Mykhailo234,Massberg Steffen15,Schulz Christian15ORCID,Orban Mathias15ORCID

Affiliation:

1. Department of Internal Medicine I, Ludwig Maximilians University, 81377 Munich, Germany

2. Laboratory for High Energy Physics (LHEP), Albert Einstein Center for Fundamental Physics, University of Bern, 3012 Bern, Switzerland

3. Theodor Kocher Institute, University of Bern, 3012 Bern, Switzerland

4. Data Science Lab, Mathematical Institute, University of Bern, 3012 Bern, Switzerland

5. DZHK (German Centre for Cardiovascular Research), Partner Site Munich Heart Alliance, 80802 Munich, Germany

Abstract

Platelets are generated by specialized cells called megakaryocytes (MKs). However, MK’s origin and platelet release mode have remained incompletely understood. Here, we established direct visualization of embryonic thrombopoiesis in vivo by combining multiphoton intravital microscopy (MP-IVM) with a fluorescence switch reporter mouse model under control of the platelet factor 4 promoter (Pf4CreRosa26mTmG). Using this microscopy tool, we discovered that fetal liver MKs provide higher thrombopoietic activity than yolk sac MKs. Mechanistically, fetal platelets were released from MKs either by membrane buds or the formation of proplatelets, with the former constituting the key process. In E14.5 c-Myb-deficient embryos that lack definitive hematopoiesis, MK and platelet numbers were similar to wild-type embryos, indicating the independence of embryonic thrombopoiesis from definitive hematopoiesis at this stage of development. In summary, our novel MP-IVM protocol allows the characterization of thrombopoiesis with high spatio-temporal resolution in the mouse embryo and has identified membrane budding as the main mechanism of fetal platelet production.

Publisher

MDPI AG

Subject

General Medicine

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