Abstract
Tumour-associated macrophages (TAMs) support cancer cell survival and suppress anti-tumour immunity. Tumour infiltration by CD163pos TAMs is associated with poor outcome in several human malignancies, including multiple myeloma (MM). Signal transducer and activator of transcription 3 (STAT3) is over-activated in human cancers, and specifically within TAMs activation of STAT3 may induce an immunosuppressive (M2-like) phenotype. Therefore, STAT3-inhibition in TAMs may be a future therapeutic strategy.
We investigated TAM markers CD163, CD206, and activated STAT3 (pSTAT3) in patients with MGUS (n = 32) and MM (n = 45), as well as healthy controls (HCs, n = 13).
Blood levels of the macrophage biomarkers sCD163 and sCD206, and circulating cytokines, as well as bone marrow mRNA expression of CD163 and CD206, were generally increased in MGUS and MM patients, compared to HCs, but to highly similar levels. By immunohistochemistry, bone marrow levels of pSTAT3 were increased specifically within CD163pos cells in both MGUS and MM patients.
In conclusion, macrophage-related inflammatory changes, including activation of STAT3, were present already at the MGUS stage, at similar levels as in MM. Specific increase in pSTAT3 levels within CD163pos cells supports that the CD163 scavenger receptor may be a useful target for future delivery of STAT3-inhibitory drugs to TAMs in MM patients.
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Introduction
Multiple myeloma (MM) is the second most common hematology malignancy, in which proliferating clonal plasma cells expand within the bone marrow, causing anaemia, osteolytic bone lesions, and hypercalcaemia. Further, monoclonal protein deposition often leads to renal failure in MM patients. Despite major advances in treatment, MM remains incurable [1].
Virtually all cases of MM are preceded by the premalignant condition monoclonal gammopathy of undetermined significance (MGUS) [2], and studies showed that the monoclonal plasma cells (mPCs) in MGUS and MM were highly similar regarding mutations, translocations, deletions, gene expression, and immunophenotype [3,4,5]. These findings have prompted researchers to look for factors outside the malignant cells, thus in the bone marrow microenvironment, in search of the key factors that drive transitioning from MGUS to MM [3, 5, 6].
The bone marrow microenvironment (the “myeloma niche”) is known to be vital for MM cell survival, and the success of the “novel agents” is partly owing to their effects on MM supportive cells [7]. Therefore, the microenvironmental changes during transition from healthy to MGUS, and from MGUS to MM, are of particular interest. Along with the MM supportive bone marrow stromal cells (BMSCs), there has been a rising interest in the role of tumour-associated macrophages (TAMs) in MM pathobiology. In most human malignancies, infiltration by TAMs is associated with poor outcome [8, 9], due to TAM-mediated resistance to chemotherapy, suppression of anti-tumour immunity, increased angiogenesis, and ultimately metastasis [10,11,12].
The paradigm of macrophage-polarization comprises two extremes: M1-like (classically activated, pro-inflammatory) and M2-like (alternatively activated, anti-inflammatory) macrophages [13]. The activation state of TAMs mostly falls within the M2-spectrum, and TAMs are thought to perform tasks similar to those of M2-like macrophages in normal physiology—e.g. in wound healing [14, 15].
In patients with MM, high bone marrow infiltration by CD163pos TAMs has been associated with poor outcome [16,17,18]. In a recent study, MM bone marrow biopsies were investigated for inducible nitric oxide synthase (iNOS) and CD163 expression to identify M1-like and M2-like TAMs, respectively. High infiltration by CD163pos (M2) cells was associated with poor outcome, whereas high infiltration with iNOSpos (M1) cells was associated with longer survival [19]. These results may be explained, at least in part, by TAM-induced resistance to anti-myeloma treatment [20, 21], as well as immunosuppressive functions of M2-like TAMs [22, 23]. In line with this, we previously showed that higher serum levels of the M2-related macrophage-derived biomarkers soluble CD163 (sCD163) and soluble mannose receptor/CD206 (sCD206), at the time of MM diagnosis, were associated with poor outcome [24, 25].
Importantly, TAMs can be “re-programmed” from M2-like towards M1-like cells, which may restore anti-tumour immunity, and thus may be a strategy for novel anti-cancer therapy [12, 23, 26, 27]. Further, in murine models of MM, macrophages could be activated to kill MM cells in vivo by blocking the anti-phagocytic protein CD47 [28], or by M1-polarizing stimuli [29, 30]. One attractive target is inhibition of the signal transducer and activator of transcription 3 (STAT3) transcription factor within TAMs [12, 31]. In several solid tumours, STAT3 is over-activated within immune cells, which has been associated with cancer-promoting functions, including suppression of anti-tumour immunity [22, 32]. Thus, inhibition of STAT3 specifically within TAM may be able to restore anti-tumour immunity [31, 33, 34].
Strategies for re-programming of TAMs are now within reach of systemic therapy owing to the development of technologies for specific targeting of drugs to macrophages, e.g. by antibody targeting of the CD163 scavenger receptor, which is highly expressed by human TAMs [13, 35,36,37].
The aim of the present study was to characterize macrophages/TAMs in a prospective cohort of patients with newly diagnosed MGUS or MM, especially regarding expression of the TAM markers CD163 and CD206. Furthermore, we examined the expression of activated (phospho-Tyr-705)-STAT3 within the bone marrow of patients with MM and MGUS — including activated STAT3 localized within CD163pos TAMs, which may be a future therapeutic target.
Materials, subjects, and methods.
Patients and collected samples
In this prospective study, we included patients with a positive M-protein measurement, that were subsequently diagnosed with MGUS (n = 32) or MM (n = 45) at the Department of Hematology, Aarhus University Hospital, Aarhus, Denmark between 2011 and 2015. Included patients diagnosed with other conditions (e.g. CLL or plasmacytoma, n = 8) were excluded from the study. In addition, we included elderly volunteers to serve as healthy controls (HCs, n = 13).
At the time of diagnosis, we collected whole bone marrow aspirate for RNA purification using the PAXgene Bone Marrow RNA system (Qiagen, Hilden, Germany) according to the manufactures instructions, to stabilize bone marrow RNA levels at sample collection. Further, at diagnosis, serum and EDTA stabilised plasma samples were collected. All samples were stored at 80 °C. For immunohistochemistry (IHC), we used the Jamshidi biopsy taken for diagnostic purpose. For eight patients, this biopsy was not available, and the diagnostic bone marrow aspirate was used for IHC.
Data on basic patient characteristics along with clinical and laboratory data, as well as bone marrow mPC infiltration determined by a pathologist, were obtained from medical records. The study was approved by the Central Denmark Region Committee on Health Research Ethics (M-20100171) and conducted according to the declaration of Helsinki. All patients and control subjects gave informed written consent before inclusion.
Serum/plasma levels of sCD163, sCD206, and inflammatory cytokines
Serum concentrations of the macrophage activation biomarkers sCD163 and sCD206 were measured using our in-house enzyme-linked immunosorbent assays (ELISA) as described in detail previously [38, 39]. Samples were run on an automated BEP 2000 system (Siemens Healthcare Diagnostics, Munich, Germany). Plasma concentrations of cytokines were measured using electro-chemo-luminescence- based multiplex sandwich immunoassays according to the manufacturer instructions (Meso Scale Discovery, Rockville, MD): Interleukin-1 beta (IL-1β), IL-6, IL-10, IL-12p70, tumour necrosis factor alpha (TNFα), and interferon gamma (IFNγ).
Reverse transcription quantitative polymerase chain reaction (RT-qPCR)
Purified RNA was reverse transcribed to cDNA in a 20 μL reaction of 2.5 μM Oligo(dT) (DNA Technology, Risskov, Denmark), 1 mM dNTP mix (VWR International, Radnor, PA), 2.5 U/μL MulV reverse transcriptase enzyme, 1 U/μL RNase inhibitors, 1 × PCR buffer and 6.25 mM MgCl2 (all from Applied Biosystems, Thermo Fisher Scientific, Waltham, MA). In each reaction, the RNA input was 100 ng (measured using a NanoDrop 2000 spectrophotometer, Thermo Fisher Scientific).
Quantitative PCR was performed on a LightCycler 480 instrument (Roche, Basel, Switzerland) in a 10 μL reaction with primers, 480 SYBR Green I Master mix (Roche), and 1μL cDNA (generated as described above). Fifty qPCR cycles were run; denaturation at 95 °C for 10 s, 20 s at annealing temperature, and 72 °C for 5 s (see Supplemental table 1 for primer sequences, concentrations, and annealing temperatures). All samples were run in duplicates. For relative mRNA quantification by RT-qPCR, a standard curve (calibrator) was included in each run (The E-Method, recommended by Roche). This compensates for variation in reaction efficiency, both day-to-day and inter-run variation. All qPCR results were normalized to the household gene SDHA (succinate dehydrogenase complex, subunit A), which was identified as the most stable of five tested household genes (Actin, HMBS, GAPDH, SDHA, YWHAZ) using the NormFinder algorithm [40]. Primers were from Eurofins Genomics (Ebersberg, Germany).
Immunohistochemistry
Sections (3 µm) of formaldehyde-fixed paraffin-embedded bone marrow samples, as well as control sections from healthy organs (pancreas, liver, and pharyngeal tonsil—included on every slide, Supplemental Fig 2), were mounted on glass slides, incubated for 1 h at 60 °C, and stored at 4 °C until use. Staining was performed on the automated platform Benchmark XT (Ventana Medical Systems, Roche Group, Tucson, AZ). The following monoclonal antibodies were used: Mouse anti-human CD163 (clone Edhu-1, dilution 1:450, Bio-Rad, Oxford, the UK), rabbit anti-human phospho-(Y705)-STAT3 (clone D3A7, dilution 1:50, Cell Signaling Technologies, Danvers, MA), mouse anti-human CD206 (clone 5C11, dilution 1:200, LSBio, Seattle, WA).
Antigen retrieval was done using cell conditioning solution 2 (CC2, Ventana Medical Systems). For the CD163/pSTAT3 double staining, additional antigen retrieval was performed using Protease 3 (Ventana Medical Systems), and lastly, Ultra Wash (Ventana Medical Systems) was used to reduce non-specific staining.
Visualization of pSTAT3 was performed with OptiView DAB (3,3’-diaminobenzidine) IHC Detection Kit, CD206 by UltraView Universal DAB Detection Kit, and CD163 by UltraView Universal Alkaline Phosphatase (AP) Red Detection Kit (all from Ventana Medical Systems). Standard haematoxylin counterstaining was done for all sections. One section from each patient/control was examined for each staining. Staining protocols were validated by a hematopathologist, including comparisons between single and double stainings for the CD163/pSTAT3 protocol showing good concordance.
Digital image analysis
Slides were digitized using a Nanozoomer 2.0HT (Hamamatsu Photonics KK, Hamamatsu City, Japan) at a magnification of 20 × in the NDPI file format. Digitized slides were analysed using Visiopharm Visiomorph (VIS) software (Version 6, Visiopharm, Hørsholm, Denmark). Using VIS software, specific application protocol packages (APPs) were developed to analyse each staining (see Fig. 3a). The results were expressed as % Area Fraction (%AF), which is the positively stained area (µm2) as % of the total analysed area (µm2) within the biopsy. Thus, an AF of 8% for CD163 denotes that 8% of the analysed area stained positive for CD163. Tissue areas were identified using the “tissue detect” function in VIS, with subsequent manual adjustment to define the final used “region of interest” (ROI), which excluded areas with bone and cartilage tissues. Using the developed APPs, we were able to detect three staining intensities for CD163 and CD206, and two intensities for pSTAT3 (more intense staining is shown by darker colours in the + APP picture in Fig. 3a.) Due to some non-specific CD206 staining, we chose to exclude CD206low areas from further analyses (this did not change the statistical results.) To quantify CD163-associated pSTAT3 signal (a measure of activated STAT3 within CD163pos cells), we instructed the CD163/pSTAT3 APP to quantify the pSTAT3 positive area that was surrounded by CD163 positive area (> 50% of pSTAT3 area surrounded, Fig. 4c).
Statistical analyses
Statistical analyses were performed using STATA version 14 for Mac OS (StataCorp LP, TX). Graphs were made using Prism 5d for Mac OS (GraphPad software, Inc., La Jolla, CA). To test differences between patient groups, we used one-way analysis of variance (ANOVA) and t-test when appropriate. Gaussian distribution of data was assessed using Q-Q plots. Data with non-normal distribution were log-transformed using the natural logarithm to obtain a normal distribution before statistical analysis. For data with significant differences in standard deviations between groups Kruskal–Wallis and Mann–Whitney (rank-sum) tests were used. A P value ≤ 0.05 was considered statistically significant.
Results
Basic characteristics of the included patients and controls with paraclinical data from the time of diagnosis are shown in Table 1. MGUS and MM patients were slightly older than the HCs (P < 0.01). Eighty percent of the MM patients had treatment demanding disease at diagnosis. Patients with MM had lower haemoglobin (P < 0.0001), and levels of both serum M-protein and bone marrow mPC infiltration were higher in MM compared to MGUS (P < 0.0001) as expected.
Increased levels of peripheral blood inflammatory markers in MGUS and MM patients
Previously, we showed in retrospective studies that higher serum levels of macrophage activation markers sCD163 and sCD206 were associated with poor overall survival in MM patients [24, 25].
In the present prospective study, levels of sCD163 and sCD206 were slightly increased in both MGUS and MM compared to HCs (Fig. 1a, not statistically significant for sCD163 in MM vs. HCs). Interestingly, there were no significant differences between MGUS and MM patients regarding both sCD163 and sCD206 levels (P > 0.2). Further, levels of sCD163 and sCD206 were positively correlated in MGUS and MM patients (P < 0.05 and < 0.0005, respectively), whereas this was not seen in HCs (P = 0.2, Supplemental Fig 1a.)
The examined cytokines showed a pattern similar to the macrophage activation markers, with significantly increased levels of TNFα, IL-1β, IL-6, IL-10 in MGUS and MM, compared to HCs, and the measured cytokine levels did not differ between MGUS and MM patients (all P > 0.2 except for TNFα (P = 0.05), Fig. 1b).
Increased gene expression of TAM markers CD163 and CD206 in MGUS and MM bone marrow
We investigated gene expression levels of CD163 and CD206 within the bone marrow microenvironment of HCs, MGUS, and MM patients by qPCR on RNA isolated from bone marrow aspirates. Both CD163 and CD206 mRNA expression were markedly higher in patients with MGUS (P < 0.001) and MM (P < 0.002) compared to HCs (Fig.2). Interestingly, CD163 and CD206 mRNA levels were increased to similar levels in MGUS and MM patients (P ≥ 0.50). Further, expression levels of CD163 and CD206 were positively correlated in both MGUS (P = 0.03) and MM patients (P < 0.0001), but not in HCs (P = 0.96, Supplemental Fig. 1b).
Bone marrow immunohistochemistry: Increased CD163 but decreased CD206 expression in MGUS patients
We also investigated protein levels of TAM markers CD163 and CD206 within the MGUS and MM bone marrow microenvironment using immunohistochemistry (IHC) with digital image analysis (Fig. 3a). Double stainings for CD163 and pSTAT3 and single stainings for CD206 were performed (Fig. 3b). Results are expressed as % Area Fraction (%AF) of positive staining relative to the total analysed area. Patients with MGUS had significantly higher CD163pos %AF compared to HC (P = 0.01), but only a tendency for higher CD163pos %AF was observed in MM patients (P = 0.12). Further, there was no significant difference in total CD163pos %AF between MGUS and MM (P = 0.06). For CD206, patients with both MGUS and MM had significantly lower %AF than HCs (P = 0.0002 and 0.01, respectively), and MM patients had slightly higher CD206%AF than in MGUS (P = 0.02).
As a measure of M2-like polarization of bone marrow macrophages, we quantified areas with “high expression” of CD163 or CD206 (the highest staining intensity as shown in Fig. 3a). This showed results similar to total CD163 and CD206 expression levels; compared to HCs, the CD163high area was significantly larger in MGUS (P < 0.05), but not in MM (P = 0.3), whereas the CD206high area was smaller in patients with MGUS compared to HCs (P < 0.001) and was larger in MM compared to MGUS patients (P = 0.01, Fig. 3c).
There was a positive correlation between CD163 and CD206 %AFs in MM patients (P = 0.03), but not for HCs (P = 0.92) or MGUS patients (P = 0.47, Supplemental Fig. 1c).
Increased bone marrow STAT3 activation within CD163pos cells in MGUS and MM patients
Bone marrow levels of activated STAT3 (by phosphorylation of Tyr-705, pSTAT3) and association with CD163pos macrophages were also examined by IHC. Overall, expression levels of pSTAT3 were not significantly higher in MGUS and MM patients, compared to HCs (P = 0.23, Fig. 4a).
However, there was a positive correlation between the expression levels of CD163 and pSTAT3 within the bone marrow biopsies (R = 0.46, P < 0.0001, Fig. 4b). Using digital image analysis, we then investigated the level of STAT3 activation specifically within CD163pos cells (quantified as CD163-associated pSTAT3 staining, Fig. 4c). Interestingly, both patients with MGUS and MM had significantly higher levels of pSTAT3 within CD163pos cells, compared to HCs (P < 0.001 and < 0.01, respectively, Fig.4d). Also, the relative amount of total pSTAT3 staining that was CD163-associated, was significantly higher in both MGUS (P < 0.0001) and MM patients (P = 0.003) compared to HCs, but also with markedly higher levels in MGUS compared to MM patients (P = 0.0001) —indicating a shift in the location of activated STAT3 towards macrophages in MM, and especially in the premalignant condition MGUS (Fig.4d).
Associations of TAM markers with MM pathophysiology and prognostic factors
There were no clear associations between the analysed TAM markers in the MM patients and bone marrow mPC infiltration, elevated LDH levels, or adverse cytogenetic profile (del(17p), t(4;14), or t(14;16), data not shown). Figure 5 shows CD163, CD206, and pSTAT3 data for the included MM patients, in relation to International Staging System (ISS) stage and bone disease severity at the time of diagnosis. Both serum sCD206 and CD206%AF tended to be higher in patients with ISS 3 (both P = 0.02), whereas pSTAT3 levels were lower in most patients with ISS 3 (P = 0.03). We also observed higher CD163 and CD206 mRNA expression in the bone marrow of patients with the most severe bone disease at diagnosis (P = 0.05 and 0.03, respectively).
Discussion
Tumour-associated macrophages are abundant in tumours, including the myeloma bone marrow microenvironment, and have attracted increasing attention in recent years due to their tumour-promoting functions. Thus, TAMs are now considered important future therapeutic targets in cancers, including MM [12, 30, 41].
Here, we describe levels of circulating macrophage-related and general inflammatory markers, as well as bone marrow microenvironment levels of TAM markers CD163, CD206, and pSTAT3, covering the range from healthy to MGUS and to MM, in a prospective study.
The main findings of the study were increased levels of TAM markers, including activated STAT3 specifically within bone marrow CD163pos cells, in both MGUS and MM patients. Further, TAM markers were increased already at the MGUS stage, both in the bone marrow and in the circulation, to levels seen in MM, which was accompanied by increased systemic cytokine levels.
Statistical power of the study could have been increased by inclusion of more healthy controls. However, it is difficult to recruit healthy volunteers who are of relatively high age, and also willing to volunteer for bone marrow and blood sampling.
It is recognized that changes within the bone marrow microenvironment of MM patients establish a “niche” with MM-protective effects [6], and TAMs are known to play important roles in MM pathobiology [16, 17, 19,20,21, 30]. Interestingly, we observed that such microenvironmental changes seemed to be established already at the premalignant MGUS stage. Thus, we found significantly increased bone marrow levels of CD163 and CD206 mRNA in both MGUS and MM, but with no difference between the two disease states. Further, we found similarly increased blood levels of sCD163 and sCD206, as well as inflammatory cytokines, for MGUS and MM patients (not statistically significant for sCD163 in MM). The similarly increased cytokine levels correspond with recently published results [42]. Previously, we reported serum levels of sCD163 and sCD206 as independent prognostic biomarkers in MM patients [24, 25], but only one report with few patients has previously compared serum levels of sCD163 in patients with MGUS and MM with HCs, showing no significant difference [43].
In the present study, IHC analysis of bone marrow CD163 and CD206 expression showed a mixed picture, with increased expression of CD163 but decreased CD206 in MGUS, and no clear changes in MM. Further, healthy controls had the highest bone marrow CD206 levels. A previous study showed increased bone marrow CD206 expression, and no significant changes in CD163 expression, in MM patients vs. non-MM patient controls with “normal bone marrow” [41]. Thus, our CD206 IHC results are in contrast to this study. We are not aware of other studies that have compared CD206 bone marrow levels between MM and MGUS patients, and with healthy controls. Thus, further studies are needed.
Numerous studies have investigated tumour CD163 expression by IHC and demonstrated associations with clinical outcome [8]. However, few studies have investigated CD163 mRNA expression in human tumours, e.g. one study showed association between high CD163 mRNA levels and poor outcome in bladder cancer [44]. The increased CD163 and CD206 bone marrow mRNA levels in both MGUS and MM have not previously been described and should be investigated further as prognostic markers.
It has been shown that genetic abnormalities characteristic for MM mPCs is also present in mPCs from MGUS patients [3, 4], indicating that changes in the bone marrow microenvironment may drive the progression from MGUS to MM [5, 6]. Thus, our findings of highly similar levels of macrophage-related inflammation in MGUS and MM are interesting, indicating that TAMs of the myeloma microenvironment may be polarized already during MGUS.
In the bone marrow biopsies, there was a strong correlation between CD163 and activated STAT3 (pSTAT3) levels. This is not surprising since STAT3 activation is known to upregulate CD163 on human macrophages [45, 46]. Some might be concerned that the used CD163/pSTAT3 double staining would favour such an association, which should be taken into account. However, as described, our assay validation showed good concordance between single/double staining. Further, we observed significantly higher levels of STAT3 activation within CD163pos cells in the bone marrow of both MGUS and MM patients compared to HCs. Interestingly, the relative amount of pSTAT3 within CD163pos cells (% of total pSTAT3) was higher in MGUS compared to both HCs and MM. The lower levels of CD163-associated pSTAT3 in MM compared to MGUS patients may seem unexpected, however, this result could be impacted by the higher infiltration in MM of mPCs that may also be pSTAT3pos. Nevertheless, STAT3 signalling in TAMs and myeloid-derived suppressor cells can induce an immunosuppressive phenotype [22, 32, 47], and this may indicate a role for macrophage STAT3 over-activation in establishing the immunosuppressive “bone marrow niche” already during the MGUS stage. Such STAT3 activation in TAMs has been proposed as a future therapeutic target [33, 34, 36], since specific STAT3 inhibition can re-program TAMs from an M2-like (pro-tumour) to an M1-like (tumouricidal) phenotype [22, 31, 32]. Recently, M2-to-M1 re-programming of macrophages showed anti-myeloma effects in vivo [30]. However, specifically in MM, functional studies demonstrating anti-tumour effects of TAM-specific STAT3 inhibition are needed.
Thus, STAT3 inhibition specifically within TAMs may be an attractive anti-cancer therapeutic strategy in several malignancies [12, 31, 33, 34]. We recently showed that a novel CD163-targeted STAT3-inhibitory liposome drug was able to inhibit STAT3 specifically in CD163pos cells, with a pro-inflammatory (re-programming) effect [36]. The present findings of significantly elevated levels of CD163-associated pSTAT3, in both MGUS and MM patients, encourage future studies on CD163-targeted STAT3-inhibition as an anti-myeloma immunomodulatory drug.
In conclusion, our data demonstrated similar inflammatory changes in MGUS and MM patients, with similar bone marrow expression of CD163, and increased levels of circulating macrophage biomarkers and cytokines. The specific increase in pSTAT3 levels within CD163pos cells supports that the CD163 scavenger receptor may be a useful gateway for drug delivery of STAT3-inhibitors to TAMs in MM.
Data availability
Data from the present study are available upon reasonable request to the corresponding author.
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Acknowledgements
The authors wish to thank Kirsten Petersen, Lene Dabelstein, Helle Ryom, Christina Sønderskov, and Gitte Brix for excellent technical assistance.
Funding
The work was supported by the Department of Clinical Biochemistry, Aarhus University Hospital, Denmark; The Faculty of Health, Aarhus University, Denmark; The Danish Cancer Research Foundation; The Cancer Foundation (Denmark), The Memorial Foundation of Max and Inge Wørzner, and by The Memorial Foundation of Eva and Henry Frænkel.
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MNA, NFA, MH, HJM contributed to conception and design. MNA, NFA, KLA, TP, BSS, HJM were involved in inclusion of patients and collection of data. MNA, NFA, KLA, AE, NA, MH, HJM contributed to analysis and interpretation of data. MNA was involved in drafting the article. NFA, KLA, AE, BSS, NA, TP, MH, HJM contributed to revising the manuscript critically. MNA, NFA, KLA, AE, BSS, NA, TP, MH, HJM were involved in approval of the version to be published.
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HJM is a minority shareholder in DeLiver Pharma that holds IP protecting the use of CD163 drug targeting. All other authors declare no conflict of interest.
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Andersen, M.N., Andersen, N.F., Lauridsen, K.L. et al. STAT3 is over-activated within CD163pos bone marrow macrophages in both Multiple Myeloma and the benign pre-condition MGUS. Cancer Immunol Immunother 71, 177–187 (2022). https://doi.org/10.1007/s00262-021-02952-1
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DOI: https://doi.org/10.1007/s00262-021-02952-1