Modulating inflammatory monocytes with a unique microRNA gene signature ameliorates murine ALS
Oleg Butovsky, … , Merit E. Cudkowicz, Howard L. Weiner
Oleg Butovsky, … , Merit E. Cudkowicz, Howard L. Weiner
Published August 6, 2012
Citation Information: J Clin Invest. 2012;122(9):3063-3087. https://doi.org/10.1172/JCI62636.
View: Text | PDF
Research Article Neuroscience

Modulating inflammatory monocytes with a unique microRNA gene signature ameliorates murine ALS

Abstract

Amyotrophic lateral sclerosis (ALS) is a progressive disease associated with neuronal cell death that is thought to involve aberrant immune responses. Here we investigated the role of innate immunity in a mouse model of ALS. We found that inflammatory monocytes were activated and that their progressive recruitment to the spinal cord, but not brain, correlated with neuronal loss. We also found a decrease in resident microglia in the spinal cord with disease progression. Prior to disease onset, splenic Ly6Chi monocytes expressed a polarized macrophage phenotype (M1 signature), which included increased levels of chemokine receptor CCR2. As disease onset neared, microglia expressed increased CCL2 and other chemotaxis-associated molecules, which led to the recruitment of monocytes to the CNS by spinal cord–derived microglia. Treatment with anti-Ly6C mAb modulated the Ly6Chi monocyte cytokine profile, reduced monocyte recruitment to the spinal cord, diminished neuronal loss, and extended survival. In humans with ALS, the analogous monocytes (CD14+CD16–) exhibited an ALS-specific microRNA inflammatory signature similar to that observed in the ALS mouse model, linking the animal model and the human disease. Thus, the profile of monocytes in ALS patients may serve as a biomarker for disease stage or progression. Our results suggest that recruitment of inflammatory monocytes plays an important role in disease progression and that modulation of these cells is a potential therapeutic approach.

Authors

Oleg Butovsky, Shafiuddin Siddiqui, Galina Gabriely, Amanda J. Lanser, Ben Dake, Gopal Murugaiyan, Camille E. Doykan, Pauline M. Wu, Reddy R. Gali, Lakshmanan K. Iyer, Robert Lawson, James Berry, Anna M. Krichevsky, Merit E. Cudkowicz, Howard L. Weiner

×

Figure 18

Identification of a unique gene signature in CD14+CD16 blood monocytes from ALS subjects.

Options: View larger image (or click on image) Download as PowerPoint
Identification of a unique gene signature in CD14+CD16– blood monocytes ...
(A) PCA analysis of the identified affected genes between sALS and fALS subjects versus healthy controls with spatial gene distribution. (B) qRT-PCR validation of 8 selected genes in an independent cohort that were the most significantly upregulated or downregulated. Relative expression in sALS and fALS against healthy controls were calculated using the 2–ΔΔCt method. Gene expression level was normalized against the geometric mean of 3 housekeeping genes (GAPDH, TUBB, and GRB2). PCRs were run in duplicate per subject. Each data point represents an individual subject. Horizontal bars denote mean of gene expression for each group. **P < 0.01, ***P < 0.001, 1-way ANOVA followed by Dunnett’s multiple-comparison post hoc test.