Summary

Akış Sitometrisi ile Sıçan Böbrek gelen Makrofagların Fenotipik Karakterizasyonu

Published: October 18, 2016
doi:

Summary

Bu yazıda fenotipik ve flow sitometri ile sıçan böbreklerden yerleşik makrofajlar kantitatif analizi için ayrıntılı bir protokol açıklar. Elde edilen lekeli hücreler aynı zamanda, böylece deneysel modelinde elde edilen bilgileri, artan hücre sıralama, gen ekspresyon analizi veya fonksiyonel çalışmalar dahil olmak üzere, başka uygulamalar için de kullanılabilir.

Abstract

There is increasing evidence suggesting the important role of inflammation and, subsequently, macrophages in the development and progression of renal disease. Macrophages are heterogeneous cells that have been implicated in kidney injury. Macrophages may be classified into two different phenotypes: classically activated macrophages (M1 macrophages), that release pro-inflammatory cytokines and promote fibrosis; and alternatively activated macrophages (M2 macrophages) that are associated with immunoregulatory and tissue-remodeling functions. These macrophage phenotypes need to be discriminated and analyzed to determine their contribution to renal injury. However, there are scarce studies reporting consistent phenotypic and functional information about macrophage subtypes in inflammatory renal disease models, especially in rats. This fact may be related to the limited macrophage markers used in rats, contrary to mice. Therefore, novel strategies are necessary to quantify and characterize the renal content of these infiltrating cells in a reliable way. This manuscript details a protocol for kidney digestion and further phenotypic and quantitative analysis of macrophages from rat kidneys by flow cytometry. Briefly, kidneys were incubated with collagenase and total macrophages were identified according to the dual presence of CD45 (leukocytes common antigen) and CD68 (PAN macrophage marker) in live cells.This was followed by surface staining of CD86 (M1 marker) and CD163 (M2 marker). Rat peritoneal macrophages were used as positive control for macrophage marker detection by flow cytometry. Our protocol resulted in low cellular mortality and allowed characterization of different intracellular and surface protein markers, thus limiting the loss of cellular integrity observed in other protocols. Moreover, this procedure allows the use of macrophages for further techniques, including cell sorting and mRNA or protein expression studies, among others.

Introduction

Renal disease is a global health problem, with increased prevalence, and associated with elevated morbidity and mortality1. One of the most important mechanisms involved in the progression and development of renal injury is inflammation, mainly triggered by macrophages. Macrophages play a pivotal role in many inflammatory diseases, including renal disorders2. Thus, an elevated presence of infiltrating macrophages has been reported in biopsies from patients with acute kidney injury (AKI) or chronic kidney disease (CKD)3,4. Recent studies suggest that the long-term outcome of renal disease could be controlled by macrophages5,6. In response to the local microenvironment, macrophages may differentiate into different phenotypes that play diverse biological functions7. Two well differentiated macrophage phenotypes have been established: classically activated macrophages (M1 macrophages) and alternatively activated macrophages (M2)8. M1 macrophages promote inflammation, whereas M2 macrophages have an anti-inflammatory role and are involved in tissue repair9. Therefore, a better knowledge of macrophage heterogeneity is necessary to understand their regulation and contribution to renal pathology and develop novel therapeutic approaches.

Both, murine and rats models have been widely used to understand the molecular and cellular mechanism involved in renal injury10. However, there are substantial differences in the diverse markers used to identify macrophages phenotypes between these rodents. Hence, several murine markers, such as F4/80 or Ly6C are not used in rats, thus limiting the extrapolation of findings between these species. Moreover, there is a limited number of markers describing macrophage phenotypes in rats, explaining the scarce studies analyzing macrophage heterogeneity in these animals as compared with mice. Therefore, new strategies for macrophage subset characterization are necessary to understand the role of macrophages in renal disease models in rats.

This manuscript describes a protocol for the phenotypic and quantitative analysis of macrophages from rat kidneys by flow cytometry. This technique can be further followed by several assays, including cell sorting and mRNA or protein expression studies to allow in-depth characterization of the role of macrophages in renal disease.

Protocol

Bu protokol Direktifi Avrupa Parlamentosu 2010/63 / AB ve Ulusal Rehber 53/2013 aşağıdaki yerel Kurumsal Hayvan Bakım ve Kullanım Komiteleri tarafından onaylandı. Reaktifler ve Çözümleri 1. Hazırlık Steril koşullar altında tüm reaktifler ve çözümler hazırlamak ve bir laminar akış başlığı altında kullanınız. 4 ° C'de çözüm tutun. lekeleme tampon maddesi hazırlanması (% 2 fetal sığır serumu 1x Dulbecco PBS (FBS)). tuzlu su, her ml kolajenaz 0….

Representative Results

Biz böbrekteki makrofajlar infiltre artan varlığı ile ilişkili renal hasar inflamatuar deneysel modelinde makrofaj heterojenite analiz. Daha önce belirtildiği gibi 12 Bu modelde, böbrek hasarı, Wistar sıçanlarının 3 hafta için içme suyu aldosteronun (1 mg -1 kg-1 gün) artı tuz (NaCl,% 1), ilaç olarak verilmesi ile indüklenmiştir. Deneylerimizde çizelgesi, Şekil 1 &…

Discussion

Makrofajlar, renal bozukluklar da dahil olmak üzere, farklı enflamatuar hastalıkların, önemli bir rol oynamaktadır, heterojen hücrelerdir. Her makrofaj ICSI'nin glomerülonefrit, diyabetik nefropati ve böbrek kanseri 14-16 belirtildiği gibi, böbrek hasarı gelişmesine farklı bir şekilde katkıda çünkü böbrek hastalığı makrofajlar alt gruplarının karakterizasyonu artan bir ilgi vardır. Akut böbrek hasarı erken evrelerinde, M1 makrofajlar bir üstünlüğü tübüler nekroz ve infla…

Disclosures

The authors have nothing to disclose.

Acknowledgements

This work was supported by grants from FIS/FEDER (Programa Miguel Servet: CP10/00479, PI13/00802 and PI14/00883), Spanish Society of Atherosclerosis, Spanish Society of Nephrology and Fundaciòn Renal Iñigo Alvarez de Toledo (FRIAT) to Juan Antonio Moreno. FIS/FEDER funds PI14/00386 and Instituto Reina Sofìa de Investigaciòn Nefrològica to Jesús Egido. Fundaciòn Conchita Rabago to Melania Guerrero Hue. Fundaciòn Renal Iñigo Alvarez de Toledo (FRIAT) to Alfonso Rubio Navarro.

Materials

Laminar flow hood Faster Or equivalent equipment
Centrifuge Hettich Or equivalent equipment
Flow cytometer (FACSAria) BD Biosciences
Fetal bovine serum BioWest S1820-500
PBS 10x LONZA BE17-515Q
Collagenase Sigma-Aldrich 12/1/9001
ACK Lysing Buffer Thermo Fisher Scientific A10492-01
Flow cytometry strainers BD Biosciences 340626
Falcon cell strainers Thermo Fisher Scientific 352340
Flow cytometry tubes Falcon 352052 5 ml Polystyrene Round-Bottom Tube
Centrifuge tubes Corning centristar 430791
Water bath Memmert GmbH + Co. KG WNE 7 37ºC
Fixation/Permeabilization Solution or Permeabilization/Wash Buffer BD Biosciences 554714
Rompum (Xylazine) Bayer Or equivalent
Ketalar (Ketamine) Pfizer Or equivalent
Hanks’ balanced salt solution Sigma-Aldrich H8264-500ML
Saline solution Braun 622415
Anti-CD45 (clone:OX-1) APC-Cy7 Biolegend 202216 Diluted 1:100
Anti-CD68 (clone: ED1) FITC Bio-RAD MCA341F Diluted 35:1000
anti-CD86 (clone: 24F) PE Biolegend 200307 Diluted 35:1000
anti-CD163 (clone: ED2) Alexa Fluor 647 Bio-RAD MCA342R Diluted 4:100
Live/dead stain  Molecular Probes L34955 Diluted 3:1000

References

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Cite This Article
Rubio-Navarro, A., Guerrero-Hue, M., Martín-Fernandez, B., Cortegano, I., Olivares-Alvaro, E., de las Heras, N., Alía, M., de Andrés, B., Gaspar, M. L., Egido, J., Moreno, J. A. Phenotypic Characterization of Macrophages from Rat Kidney by Flow Cytometry. J. Vis. Exp. (116), e54599, doi:10.3791/54599 (2016).

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