Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis
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2016
Authors
Vignjević-Petrinović, Sanja
Budeč, Mirela

Marković, Dragana

Gotić, Mirjana
Mitrović-Ajtić, Olivera

Mojsilović, Slavko

Stošić-Grujičić, Stanislava
Ivanov, Milan

Jovčić, Gordana
Čokić, Vladan

Article (Published version)

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Macrophage migration inhibitory factor is a well-known proinflammatory cytokine that is released during systemic stress response. Although MIF can affect erythrocyte production, the role of this cytokine in stress-induced erythropoiesis is completely unknown. To extend our previous findings showing that chronic psychological stress stimulates extramedullary erythropoiesis, here we examined whether MIF is involved in the control of stress-induced erythropoietic response. Adult male C57BL/6 wild-type (WT) and MIF-KO (knock-out) mice were subjected to 2-h daily restraint stress for either 7 or 14 consecutive days. The number of erythroid progenitors and CD71/Ter119 profile of erythroid precursors were analyzed in the bone marrow and spleen. Additionally, MIF protein expression was assessed in WT mice. Our results demonstrated that chronic restraint stress enhanced the number of both erythroid progenitors and precursors in the spleen. Stress-induced increase in the number of splenic late e...rythroid progenitors as well as in the percentage of CD71(+)Ter119(+)-double-positive precursors was significantly more pronounced in MIF-KO mice compared to WT animals. Furthermore, repeatedly stressed WT animals demonstrated an augmented MIF expression in the spleen. Unlike the spleen, the bone marrow of chronically stressed WT mice exhibited less prominent changes in erythropoietic stress response and no significant alteration in MIF expression. In addition, MIF deficiency did not influence the bone marrow erythropoiesis in stressed animals. These findings suggest that MIF regulates extramedullary erythropoiesis by inhibiting an overexpansion of splenic immature erythroid cells during chronic stress and indicate a novel role for this cytokine under chronic stress conditions.
Keywords:
MIF / Erythropoiesis / Stress / Spleen / Bone marrowSource:
Histochemistry & Cell Biology, 2016, 146, 3, 311-324Publisher:
- Springer, New York
Funding / projects:
DOI: 10.1007/s00418-016-1442-7
ISSN: 0948-6143
PubMed: 27129368
WoS: 000382043300008
Scopus: 2-s2.0-84964621678
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Institut za medicinska istraživanjaTY - JOUR AU - Vignjević-Petrinović, Sanja AU - Budeč, Mirela AU - Marković, Dragana AU - Gotić, Mirjana AU - Mitrović-Ajtić, Olivera AU - Mojsilović, Slavko AU - Stošić-Grujičić, Stanislava AU - Ivanov, Milan AU - Jovčić, Gordana AU - Čokić, Vladan PY - 2016 UR - http://rimi.imi.bg.ac.rs/handle/123456789/745 AB - Macrophage migration inhibitory factor is a well-known proinflammatory cytokine that is released during systemic stress response. Although MIF can affect erythrocyte production, the role of this cytokine in stress-induced erythropoiesis is completely unknown. To extend our previous findings showing that chronic psychological stress stimulates extramedullary erythropoiesis, here we examined whether MIF is involved in the control of stress-induced erythropoietic response. Adult male C57BL/6 wild-type (WT) and MIF-KO (knock-out) mice were subjected to 2-h daily restraint stress for either 7 or 14 consecutive days. The number of erythroid progenitors and CD71/Ter119 profile of erythroid precursors were analyzed in the bone marrow and spleen. Additionally, MIF protein expression was assessed in WT mice. Our results demonstrated that chronic restraint stress enhanced the number of both erythroid progenitors and precursors in the spleen. Stress-induced increase in the number of splenic late erythroid progenitors as well as in the percentage of CD71(+)Ter119(+)-double-positive precursors was significantly more pronounced in MIF-KO mice compared to WT animals. Furthermore, repeatedly stressed WT animals demonstrated an augmented MIF expression in the spleen. Unlike the spleen, the bone marrow of chronically stressed WT mice exhibited less prominent changes in erythropoietic stress response and no significant alteration in MIF expression. In addition, MIF deficiency did not influence the bone marrow erythropoiesis in stressed animals. These findings suggest that MIF regulates extramedullary erythropoiesis by inhibiting an overexpansion of splenic immature erythroid cells during chronic stress and indicate a novel role for this cytokine under chronic stress conditions. PB - Springer, New York T2 - Histochemistry & Cell Biology T1 - Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis EP - 324 IS - 3 SP - 311 VL - 146 DO - 10.1007/s00418-016-1442-7 UR - conv_3833 ER -
@article{ author = "Vignjević-Petrinović, Sanja and Budeč, Mirela and Marković, Dragana and Gotić, Mirjana and Mitrović-Ajtić, Olivera and Mojsilović, Slavko and Stošić-Grujičić, Stanislava and Ivanov, Milan and Jovčić, Gordana and Čokić, Vladan", year = "2016", abstract = "Macrophage migration inhibitory factor is a well-known proinflammatory cytokine that is released during systemic stress response. Although MIF can affect erythrocyte production, the role of this cytokine in stress-induced erythropoiesis is completely unknown. To extend our previous findings showing that chronic psychological stress stimulates extramedullary erythropoiesis, here we examined whether MIF is involved in the control of stress-induced erythropoietic response. Adult male C57BL/6 wild-type (WT) and MIF-KO (knock-out) mice were subjected to 2-h daily restraint stress for either 7 or 14 consecutive days. The number of erythroid progenitors and CD71/Ter119 profile of erythroid precursors were analyzed in the bone marrow and spleen. Additionally, MIF protein expression was assessed in WT mice. Our results demonstrated that chronic restraint stress enhanced the number of both erythroid progenitors and precursors in the spleen. Stress-induced increase in the number of splenic late erythroid progenitors as well as in the percentage of CD71(+)Ter119(+)-double-positive precursors was significantly more pronounced in MIF-KO mice compared to WT animals. Furthermore, repeatedly stressed WT animals demonstrated an augmented MIF expression in the spleen. Unlike the spleen, the bone marrow of chronically stressed WT mice exhibited less prominent changes in erythropoietic stress response and no significant alteration in MIF expression. In addition, MIF deficiency did not influence the bone marrow erythropoiesis in stressed animals. These findings suggest that MIF regulates extramedullary erythropoiesis by inhibiting an overexpansion of splenic immature erythroid cells during chronic stress and indicate a novel role for this cytokine under chronic stress conditions.", publisher = "Springer, New York", journal = "Histochemistry & Cell Biology", title = "Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis", pages = "324-311", number = "3", volume = "146", doi = "10.1007/s00418-016-1442-7", url = "conv_3833" }
Vignjević-Petrinović, S., Budeč, M., Marković, D., Gotić, M., Mitrović-Ajtić, O., Mojsilović, S., Stošić-Grujičić, S., Ivanov, M., Jovčić, G.,& Čokić, V.. (2016). Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis. in Histochemistry & Cell Biology Springer, New York., 146(3), 311-324. https://doi.org/10.1007/s00418-016-1442-7 conv_3833
Vignjević-Petrinović S, Budeč M, Marković D, Gotić M, Mitrović-Ajtić O, Mojsilović S, Stošić-Grujičić S, Ivanov M, Jovčić G, Čokić V. Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis. in Histochemistry & Cell Biology. 2016;146(3):311-324. doi:10.1007/s00418-016-1442-7 conv_3833 .
Vignjević-Petrinović, Sanja, Budeč, Mirela, Marković, Dragana, Gotić, Mirjana, Mitrović-Ajtić, Olivera, Mojsilović, Slavko, Stošić-Grujičić, Stanislava, Ivanov, Milan, Jovčić, Gordana, Čokić, Vladan, "Macrophage migration inhibitory factor is an endogenous regulator of stress-induced extramedullary erythropoiesis" in Histochemistry & Cell Biology, 146, no. 3 (2016):311-324, https://doi.org/10.1007/s00418-016-1442-7 ., conv_3833 .