Article Text
Abstract
Objective Hepatocellular carcinoma (HCC) is increasingly associated with non-alcoholic steatohepatitis (NASH). HCC immunotherapy offers great promise; however, recent data suggests NASH-HCC may be less sensitive to conventional immune checkpoint inhibition (ICI). We hypothesised that targeting neutrophils using a CXCR2 small molecule inhibitor may sensitise NASH-HCC to ICI therapy.
Design Neutrophil infiltration was characterised in human HCC and mouse models of HCC. Late-stage intervention with anti-PD1 and/or a CXCR2 inhibitor was performed in murine models of NASH-HCC. The tumour immune microenvironment was characterised by imaging mass cytometry, RNA-seq and flow cytometry.
Results Neutrophils expressing CXCR2, a receptor crucial to neutrophil recruitment in acute-injury, are highly represented in human NASH-HCC. In models of NASH-HCC lacking response to ICI, the combination of a CXCR2 antagonist with anti-PD1 suppressed tumour burden and extended survival. Combination therapy increased intratumoural XCR1+ dendritic cell activation and CD8+ T cell numbers which are associated with anti-tumoural immunity, this was confirmed by loss of therapeutic effect on genetic impairment of myeloid cell recruitment, neutralisation of the XCR1-ligand XCL1 or depletion of CD8+ T cells. Therapeutic benefit was accompanied by an unexpected increase in tumour-associated neutrophils (TANs) which switched from a protumour to anti-tumour progenitor-like neutrophil phenotype. Reprogrammed TANs were found in direct contact with CD8+ T cells in clusters that were enriched for the cytotoxic anti-tumoural protease granzyme B. Neutrophil reprogramming was not observed in the circulation indicative of the combination therapy selectively influencing TANs.
Conclusion CXCR2-inhibition induces reprogramming of the tumour immune microenvironment that promotes ICI in NASH-HCC.
- hepatocellular carcinoma
- immunotherapy
- nonalcoholic steatohepatitis
Data availability statement
Data are available in a public, open access repository. All data will be deposited with accession codes, unique identifiers or web links for publicly available datasets provided before publication.
This is an open access article distributed in accordance with the Creative Commons Attribution 4.0 Unported (CC BY 4.0) license, which permits others to copy, redistribute, remix, transform and build upon this work for any purpose, provided the original work is properly cited, a link to the licence is given, and indication of whether changes were made. See: https://creativecommons.org/licenses/by/4.0/.
Statistics from Altmetric.com
Significance of this study
What is already known on this subject?
Immune checkpoint inhibition (ICI) therapy is emerging as a promising new therapy for the treatment of advanced hepatocellular carcinoma (HCC).
Only a minority of HCC patients will respond to ICI therapy and recent data suggest that HCC on the background of non-alcoholic steatohepatitis (NASH) may have reduced sensitivity to this treatment strategy.
Neutrophils are a typical myeloid component of the liver in NASH and are found either within the HCC tumour microenvironment or in a peritumoural location.
Neutrophils have considerable phenotypic plasticity and can exist in both tumour promoting and tumour suppressing states.
Neutrophils may have the ability to influence ICI therapy.
Significance of this study
What are the new findings?
CXCR2+ neutrophils are found in human NASH and within the tumour of both human and mouse models of NASH-HCC.
The resistance of NASH-HCC to anti-PD1 therapy is overcome by co-treatment with a CXCR2 small molecule inhibitor, with evidence of reduced tumour burden and extended survival.
Anti-PD1 and CXCR2 inhibitor combine to selectively reprogramme tumour-associated neutrophils (TANs) from a protumour to an anti-tumour phenotype.
Reprogrammed TANs proliferate locally within Granzyme B+ immune clusters that contain physically associating CD8+ T cells and antigen presenting cells.
Conventional XCR1+ dendritic cells are found to be elevated in anti-PD1 and CXCR2 inhibitor treated HCCs and together with CD8+ T cells are required for therapeutic benefit.
How might it impact on clinical practice in the foreseeable future?
TANs can be selectively manipulated to adopt an anti-tumour phenotype which unlocks their potential for cancer therapy. The ability of CXCR2 antagonism to combine with ICI therapy to bring about enhanced therapeutic benefit in NASH-HCC (and potentially in HCC of other aetiologies) warrents clinical investigation.
Introduction
Primary liver cancer is emerging globally as one of the most common and deadly malignancies with 905 000 new diagnosed cases and 830 000 deaths recorded in 2020.1 Hepatocellular carcinoma (HCC) accounts for up to 85% of primary liver cancers and develops on the background of chronic liver disease caused by persistent virological (hepatitis B virus (HBV) and hepatitis C virus (HCV)) or non-virological liver damage. Due to the increasing prevalence of obesity and the metabolic syndrome a high proportion of HCC is now attributed to non-alcoholic steatohepatitis (NASH), identified as the most common risk factor for HCC in UK and USA.2 3
Possible curative options for HCC such as tumour resection, liver transplant or ablation are at present limited to a minority of patients who are diagnosed at an early stage of the disease.4 For more advanced HCC, approved systemic therapies include multikinase inhibitors and agents targeting vascular endothelial growth factor (VEGF) . More recently, immune checkpoint inhibition (ICI) has emerged as a therapeutic modality in HCC with PD1 antibodies (nivolumab and pembrolizumab) being approved, and a combination of anti-PDL1 (atezolizumab) with anti-VEGF (bevacizumab) now being first-line treatment for advanced HCC.5–7 However, only a minority (up to 30%) of HCC patients respond to immunotherapy.5–8 Moreover, it was recently reported that HCC on the background of NASH is less responsive to immunotherapy due to a NASH-induced alteration in the immune components of the liver and in particular an expansion in numbers of exhausted CD8+PD1+ T cells, that appear to promote, rather than suppress, NASH-HCC.9 10 Therefore, advanced therapeutic strategies for HCC will require a deeper appreciation of the complex immune landscape of the tumour microenvironment, and in particular, should also take into account the influence that the background liver pathology may have on the numbers, regional distributions, phenotypes and activities of key immune cell types of relevance to cancer growth.
Recent use of imaging mass cytometry (IMC) and single cell sequencing to probe the cellular constituents of human HCC revealed considerable heterogeneity within the tumour microenvironment with intratumoural region-specific distributions of immune cells.11 Regions with evidence of less aggressive cancer and ongoing liver damage (fibrogenesisis) were enriched for CD8+ T cells, B cells and CD11b+CD15+GranzymeB+ neutrophils. When considering the growing evidence for both pro-tumour and anti-tumour functions for neutrophils in a variety of cancers12 13 including HCC14 we were interested to determine if modulation of neutrophil biology within the tumour microenvironment would influence the resistance of NASH-HCC to anti-PD1 immunotherapy.
Here, we determined that the CXC chemokine receptor, CXCR2 is almost exclusively located on neutrophils in human and mouse NASH-HCC. This finding led us to ask if antagonism of CXCR2 can combine with anti-PD1 to overcome resistance of NASH-HCC to immunotherapy. Our findings suggest that this combination therapy reprogrammes the phenotype of tumour neutrophils and enhances their association with CD8+ T cells and conventional dendritic cells (cDC). Reshaping the tumour immune microenvironment was associated with a T cell- and DC-dependent reduction in tumour burden and increased survival. We propose that combined neutrophil phenotype modification and ICI may achieve improved outcomes in NASH-HCC.
Protumour CXCR2+ neutrophils associate with NASH-HCC resistance to anti-PD1 immunotherapy
To investigate the immunological determinants of unresponsiveness of NASH-HCC to anti-PD1 therapy we designed an orthotopic mouse model using the Hep-53.4 HCC cell line, which was selected due to its high mutational burden (online supplemental figure 1A–C). On the background of steatosis induced by a modified diet of high sugar and fat, we observed weight gain and larger tumours compared with non-steatotic controls (online supplemental figure 1D,E). Tumours in non-steatotic controls were responsive to anti-PD1 therapy, however, anti-PD1 showed no benefit on tumour burden, survival, steatosis, proliferation or immune cell infiltration in steatotic mice (figure 1A–F and online supplemental figure 1H,K). For an additional autochthonous model, we employed either Diethylnitrosamine (DEN) alone or in combination with the American lifestyle induced obesity syndrome diet (DEN/ALIOS), the latter to establish HCC on a background of NASH15 16 (online supplemental figure 1I–O). Anti-PD1 responsiveness was observed in DEN mice fed a control diet, whereas anti-PD1 therapy had no effect on tumour burden, proliferation, or steatosis and animal survival when mice were fed the ALIOS diet (figure 1G–L and online supplemental figure 1P,Q). However, F4/80+ and CD3+ immune cell infiltrates were increased in anti-PD1 treated ALIOS fed mice (online supplemental figure 1R,S) indicative of anticipated alterations in tumour immunity.
Supplemental material
Although elevated numbers of circulating neutrophils are associated with reduced HCC survival,17 by contrast an enrichment of tumour-associated neutrophils (TANs) is reported to correlate with improved survival.18 This latter observation indicates a potential for TANs to influence the progression of HCC and raises the question of whether immunotherapy is influencing TANs (and vice versa). Ly6G+ neutrophils were found to be present in both tumour and non-tumour tissue of orthotopic-HCC mice and were significantly elevated in both compartments in the presence of NASH and remained high with anti-PD1 therapy (figure 2A and online supplemental figure 2A). Increased numbers of TANs were also a feature in the DEN/ALIOS model and the increase reached significance with anti-PD1 treatment (figure 2B and online supplemental figure 2A). In addition, TANs were elevated in choline deficient-high fat diet (CD-HFD) spontaneous NASH-HCC model, and were retained with anti-PD1 therapy which is reported to also fail in this model9 (online supplemental figure 2B,C). Thus, we consistently observe TANs to accumulate in NASH-HCC, independent of the model examined, and they are retained in the tumour with anti-PD1 therapy. TANs display functional heterogeneity including anti-tumour or protumour phenotypes that impact on tumour growth.19 Using transcriptomic profiling of tumour-isolated Ly6G+ cells, we determined the phenotype of TANs from DEN/ALIOS tumours. To account for environmentally induced differences in gene expression,20 we compared TANs with peripheral blood and liver neutrophils. DEGs with increased expression were enriched for process networks associated with inflammatory (eg, Nfkb1/Rel, Mapk8/Jnk1, Mapk9/Jnk2, Icam1) and calcium (eg, Itpr1, Plcb1, Plcg1) signalling (figure 2C and online supplemental figure 2D). Genes associated with a protumour neutrophil phenotype, including Csf1, Ccl3, Vegfa and Ptgs2 19–21 were also significantly upregulated in TANs (online supplemental figure 2E).
Transcriptomic analysis of DEN/ALIOS tumours identified an upregulation of myeloid associated cytokine and chemokine gene expression compared with normal liver (figure 2D). Notably, ligands (Cxcl1, Cxcl2, Cxcl3, Cxcl5) for the chemokine receptor CXCR2, the latter identified as being predominantly expressed by Ly6G+ neutrophils, were all increased in tumour tissue (figure 2D,E and online supplemental figure 2F). In situ hybridation analysis of Cxcr2 expression in DEN/ALIOS mouse tumours confirmed expression of Cxcr2 to be specifically associated with morphologically identified infiltrating neutrophils and absent in parenchymal and tumour cells (figure 2F). This identifies CXCR2 as a neutrophil chemokine receptor that could be targeted to manipulate TANs in models of HCC-NASH.14 In humans, the CXCR2 ligands CXCL1 and CXCL8 were significantly upregulated in NASH-HCC compared with NASH (online supplemental figure 2G). Neutrophil chemotaxis/migratory gene ontology terms were enriched in advanced human NASH (F4 fibrosis)22 and numbers of hepatic CD66b+ neutrophils increased with severity of NASH (online supplemental figure 2H,I). Moreover, in HCC patient tissue, CD66b+ neutrophils and CXCR2+ cells predominantly localised to NASH-HCC tumours with expression of the two markers correlating, and furthermore being demonstrated to be colocalised at the cellular level (figure 2G,H and online supplemental figure 2J,K). Similar to the mouse models, CXCR2 expression was limited to infiltrating immune cells and was absent on tumour epithelium within HCC in patients (figure 2I). We additionally noted that neutrophil expression signatures were enriched in human NASH-HCC compared with HBV-HCC, HCV-HCC and alcohol-related-HCC23 (figure 2J). Thus, tumour infiltration of CXCR2-expressing neutrophils is characteristic of both murine models and human NASH-HCC and associates with resistance to anti-PD1 therapy in experimental models of NASH-HCC.9
CXCR2 antagonism resensitises NASH-HCC to immunotherapy
We next determined the effects of a CXCR2 small molecule inhibitor (AZD5069)24 in experimental NASH-HCC either administered alone or in combination with anti-PD1. We hypothesised that AZD5069 would suppress hepatic neutrophil recruitment. This was confirmed in the context of DEN-induced acute liver damage (online supplemental figure 3A–C). We also observed no change in F4/80+ macrophages and CD3+ T cells (online supplemental figure 3D,E). These data are consistent with previous studies showing that in acute inflammatory settings CXCR2 inhibition selectively reduces neutrophil recruitment.24
Treatments using either or both AZD5069/anti-PD1 were then investigated for their ability to suppress tumour growth in the DEN-ALIOS model (figure 3A). Tumour burden at day 284 was reduced for AZD5069 monotherapy and with combined AZD5069/anti-PD1 treatment compared with vehicle and anti-PD1 monotherapy, however, no change in tumour number was identified suggesting a suppression of cancer progression (figure 3B and online supplemental figure 3F,G). Examination of tumours revealed reduced numbers of epithelial mitotic bodies and a lower tumour-stage grading for the AZD5069/anti-PD1 group compared with other treatment arms including AZD5069 monotherapy without significantly altering the underlying NASH pathology (figure 3C–F and online supplemental figure 3H). This is clinically relevant as a high mitotic index in human HCC is a predictor of shorter disease-specific survival.25 It was therefore noteworthy that the combination of AZD5069/anti-PD1 improved survival relative to monotherapies (figure 3G) Importantly, the benefits of AZD5069/anti-PD1 therapy were recapitulated in the orthotopic NASH-HCC model (figure 3H–J). In contrast to the DEN/ALIOS model, a lack of therapeutic effect was observed with either AZD5069 or anti-PD1 monotherapy (figure 3I,J). However, AZD5069/anti-PD1 combination therapy reduced tumour burden at day 28 and extended survival relative to vehicle control and monotherapies (figure 3I,J and online supplemental figure 3I). Notably, the treatments had no influence on steatosis or body weight (online supplemental figure 3J,K). AZD5069/anti-PD1 treated mice reached clinical endpoint later, at which point tumour burden was similar between treatment arms, this being consistent with suppression of tumour growth (online supplemental figure 3L). Hence, although CXCR2 antagonism alone delivered modest model-dependant antitumour benefit, similar to observations made in models of non-hepatic cancers,26–31 we show that CXCR2 inhibition sensitises to anti-PD1 immunotherapy in models of NASH-HCC that are otherwise resistant to anti-PD1 monotherapy.
AZD5069/anti-PD1 therapy promotes an antitumour immune microenvironment
To further examine the concept that CXCR2 antagonism sensitises NASH-HCC to anti-PD1 therapy we asked if combination therapy activates classic T-cell mediated anti-tumour immunity. Characterisation of intratumoural T cells revealed intratumoural CD8+ T cells were significantly increased in both anti-PD1 and AZD5069/anti-PD1 therapy groups, with only anti-PD1 monotherapy significantly affecting CD4+ T cells (figure 4A and online supplemental figure 4A). Combination therapy also enhanced intratumoural CD8+ T cell numbers in the orthotopic model (online supplemental figure 4B) Flow cytometric analysis revealed no gross phenotypic changes in early effector CD8+CD44Hi T cells across treatment groups. However, anti-PD1 treatment alone significantly increased numbers of CD8+PD1+ T cells, this effect being recently reported by Pfister et al 9 who suggested this T cell phenotype compromises the efficacy of anti-PD1 treatment in NASH-HCC (online supplemental figure 4C). The percentage of CD4+PD1+ T cells was also higher in the context of anti-PD1 monotherapy relative to other treatment groups (online supplemental figure 4D). RNAseq on isolated CD3+ cells revealed enhanced expression of the recently identified T cell ageing markers Gzmk and Eomes following anti-PD1 therapy, both of which were suppressed when AZD5069 was combined with anti-PD1 (figure 4B). Alongside these changes, AZD5069/anti-PD1 therapy enhanced the expression of Granzyme B (Gzmb), a cytotoxic serine protease expressed by neutrophils, NK cells and by recently activated CD8+ T cells and for which expression correlates with clinical outcome in PD1 immunotherapy.32–35 Immunostaining of DEN/ALIOS tumours revealed that Gzmb was detected at low levels in vehicle and monotherapy groups yet in the context of AZD5069/anti-PD1 combination therapy was highly expressed and was localised within discrete immune cell clusters containing banded immature neutrophils and lymphocytes (figure 4C and online supplemental figure 4E). Enhanced Gzmb protein expression was also achieved with combination therapy in orthotopic tumours where we also noted that anti-PD1 monotherapy depressed expression of the protease relative to vehicle control (online supplemental figure 4F). These data led us to ask if depletion of CD8+ T cells would modulate the anti-tumour effects of AZD5069/anti-PD1 therapy. Depletion of CD8+ T cells was carried out by administration of anti-CD8α to mice bearing an orthotopic NASH-HCC tumour and alongside AZD5069/anti-PD1 treatment (figure 4D). Succesful depletion of CD8+ T cells was confirmed by an increase in the proportion of CD4+ cells relative to the total CD3+ population (online supplemental figure 4G–I) and resulted in a higher orthotopic tumour burden compared with IgG controls (figure 4E). The requirement for CD8+ T cells for the anti-tumour effect of combination therapy was additionally confirmed by performing anti-CD8α-mediated depletion in tumour-bearing DEN/ALIOS mice treated with combination AZD5069/anti-PD1 (online supplemental figure 4J–M).
As recruitment and activation of XCR1+ cDC1 in tumours is considered critical for activation of cytotoxic CD8+ T cells and immunotherapy36 we next assessed CD86 surface expression as a marker of cDC1 activation in mice treated with AZD5069/anti-PD1 therapy. Anti-PD1 alone had no effect on activation of intratumour XCR1+ cDC1 cells compared with vehicle controls in the DEN/ALIOS model (figure 4F). AZD5069 alone also had no effect on activation of intratumour XCR1+ cDC1 cells, likely due to the limited expression of CXCR2 on cDCs (figure 2E). However, combined AZD5069/anti-PD1 therapy substantially increased the activation of intratumoural cDC1 cells (figure 4F). As several CC chemokines associated with DC recruitment were expressed in mouse NASH-HCC tumours responding to mono and dual therapies (online supplemental figure 5A) we next determine the effects of perturbing DC recruitment employing mice that are deficient for Ccr1, Ccr2, Ccr3 and Ccr5, termed iCCR.37 These mice were treated as per the DEN/ALIOS model and AZD5069/anti-PD1 or control therapy administered (figure 4G). The number of cDC1 and cDC2 cells, and to a lesser extent F4/80+ macrophages but not neutrophils, were decreased in the tumours of iCCR mice (online supplemental figure 5B–D). Importantly, loss of myeloid recruitment alone in iCCR mice had no impact on tumour burden in the DEN/ALIOS model (figure 4H). However, unlike in wild-type mice, AZD5069/anti-PD1 therapy failed to reduce tumour burden in iCCR mice (figure 4H). This loss of effect was associated both with a reduction in tumour associated CD3+CD8+ T cells and loss of granzyme B+ immune clusters (figure 4I.J). To corroborate these data and to more specifically address the role of XCR1+ cDC1 cells we determined if AZD5069/anti-PD1 therapy of orthotopic NASH-HCC would be affected by anti-XCL1-mediated blockade of XCL1, a major chemokine involved in mediating cDC1 and CD8 T cell interactions (figure 4K).38 AZD5069/anti-PD1 therapy resulted in an increase in activated intratumoural XCR1+ cDC1 cells in line with observations in DEN/ALIOS mice, but with cDC1 activation being selectively suppressed on treatment with anti-XCL1 (online supplemental figure 5E,F). This effect was associated with loss of the anti-tumoural action of AZD5069/anti-PD1 therapy; demonstrated by increased tumour burden in anti-XCL1 treated mice compared with IgG controls (figure 4L). Confirming an associated impact on cytotoxic T cells, AZD5069/anti-PD1-induced increases in intratumoural cytotoxic CD8+ and GzmB+ cells which was suppressed when cDC1 activation was selectively blocked by anti-XCL1 (figure 4M,N). We conclude that combined suppression of CXCR2 and PD1 stimulates both intratumoural recruitment and activation of cDC1 cells enabling T cell-mediated cytotoxicity.
AZD5069/anti-PD1 therapy promotes tumour neutrophil accumulation and the formation of intratumoural immunological hubs
Given that CXCR2 is almost exclusively expressed on neutrophils (figure 2E), we were curious as to their role in AZD5069/anti-PD1 therapy and its associated tumour immune cell remodelling. Unexpectedly, we observed that combination therapy in both models of NASH-HCC was associated with a dramatic increase in TANs, whereas AZD5069 monotherapy brought about the anticipated reduction in TANs (figure 5A,B and online supplemental figure 6A). Real-time analysis of tumour neutrophil infiltration was not possible across the therapy time-course, so instead we examined circulating neutrophils sampled weekly from peripheral blood. Anti-PD1 alone had no demonstrable effects on circulating neutrophil numbers across the treatment period, whereas AZD5069 stimulated a transient increase in circulating Ly6G+ neutrophils peaking at 4 weeks after start of treatment (online supplemental figure 6B). A similar transient increase in circulating neutrophils was observed in AZD5069/anti-PD1 treated mice, however, this effect was delayed peaking at 6 weeks from start of treatment. These peripheral blood data indicated a change in neutrophil behaviour in response to dual long-term targeting of CXCR2 and PD1.
Immunohistochemical analysis of tumours identified clusters of TANs that were unique to AZD5069/anti-PD1 treatment and comprising a mixed population of banded and segmented neutrophil populations (figure 5B,C and online supplemental figure 6C). The presence of these clustered TANs in AZD5069/anti-PD1 treated HCCs was intriguing and suggestive of local proliferation. Zhu et al 39 recently described early unipotent neutrophil progenitors (NeP) that produce neutrophils from adult bone marrow (BM). Conspicuously, NePs were significantly increased not only in the BM but also in tumours of AZD5069/anti-PD1 treated mice (figure 5D and online supplemental figure 6D,E). AZD5069/anti-PD1 treatment, therefore, alters granulopoiesis, while intratumour NePs may locally generate neutrophils, thus offering an explanation for the unexpectedly elevated numbers of TANs observed in mice receiving combination therapy.
To validate the presence of immature neutrophils in combined AZD5069/anti-PD1 treated tumours we used IMC of tumour sections from DEN/ALIOS treatment arms (online supplemental figure 6F–J). Neutrophils, both immature and mature, were identified as expressing the primary granule protein MPO. We confirmed intratumoural clusters of proliferating MPO+Ki67+ neutrophils to be significantly increased in AZD5069/anti-PD1 treated mice compared with monotherapies and vehicle controls (figure 5E,F). IMC neighbourhood analysis revealed intimate associations of MPO+Ki67+ neutrophils with CD8+ T cells and MHC Class II+ (MHCII+) antigen presenting cells (APCs) that were found in the regions of interest with six out of seven AZD5069/anti-PD1 treated tumours that were examined by IMC (figure 5G–I). In contrast, for anti-PD1 and AZD5069 monotherapies, IMC only detected these mixed immune cell hubs in one tumour for each type of treatment (figure 5I).
Intravital microscopy confirmed the presence of stable tumour-associated Ly6G+ clusters, in vivo, in AZD5069/anti-PD1 treated mice (online supplemental figure 6K,L). Directly interacting Ly6G+ TANs and CD3+CD8+ T cells that maintained physical contact over several minutes or more were also observed (online supplemental figure 6M).
Longitudinal imaging of ex vivo precision cut liver slices (PCLS) was then performed to further interrogate Ly6G+ cell (neutrophil), CD8+ cell (T cell) and CD11c+ cell (DC and a subset of macrophages) dynamics within the tumours of DEN/ALIOS mice (online supplemental figure 6N,O and video). PCLS from AZD5069/anti-PD1 treated mice had the expected, elevated numbers of neutrophils, CD11c+ cells and CD8+ T cells (online supplemental figure 6P–R). Although T cell speeds remained low in PCLS from all groups, neutrophil speed was increased in AZD5069/anti-PD1 treated tumours suggesting a more actively migrating phenotype for these neutrophils (online supplemental figure 6S,T). Neutrophil-CD11c+ cell interactions were high in tumours irrespective of treatment, however, neutrophil-CD8+ T cell and CD11c+-CD8+ T cell interactions were elevated in AZD5069/anti-PD1 treated tumours compared with vehicle controls (online supplemental figure 6U–Y, video). These data provide evidence that combined therapeutic targeting of CXCR2+ neutrophils and the PD1-PDL1 immune checkpoint remodels the NASH-HCC tumour immune microenvironment, including the generation of locally proliferating immature NeP in close physical association with cytotoxic T cells.
Supplementary video
AZD5069/anti-PD1 combination therapy reprogrammes the TAN phenotype
Given that our observations were consistent with intratumoural granulopoiesis in response to combination AZD5069/anti-PD1 therapy, we more closely characterised the TAN phenotype under these conditions. Grieshaber-Bouyer et al 40 recently reported a chronologically ordered developmental path for neutrophils termed ‘neutrotime’. This extends from immature preneutrophils (early neutrotime) that are predominantly found in BM to fully mature neutrophils (late neutrotime) mainly located in the circulation and spleen (online supplemental figure 7A). TAN transcriptome analysis revealed that AZD5069/anti-PD1 therapy induced neutrotime reprogramming along this neutrotime spectrum (figure 6A and online supplemental figure 7B). TANs in vehicle, anti-PD1 and AZD5069 treated tumours phenotypically resembled mature neutrophils, expressing genes characteristic of the late neutrotime (eg, Jund, Csf3r, Rps27) (figure 6A and online supplemental figure 7B). However, late neutrotime genes were comprehensively downregulated in TANs from AZD5069/anti-PD1 treated mice, with a corresponding upregulation of transcripts characteristic of the early neutrotime (eg, Mmp8, Retnlg, Ltf, Lcn2, Camp, Chil3, Tuba1b, Fcnb). Lactoferrin (Ltf) was of particular interest among the early neutrotime genes as its protein has well documented anti-cancer activities; including the activation of DCs and macrophages and enhancing the cytotoxic properties of natural killer cells.41–43 Staining for Lactoferrin in DEN/ALIOS tumours was elevated in AZD5069/anti-PD1 treated mice where the protein was localised to the neutrophil-rich immune clusters that included banded immature neutrophils (figure 6B,C). These observations indicate a potential mechanism by which reprogrammed TANs may network with other immune cells to enact antitumoural effects.
Interrogation of transcriptome data from NASH-related and non-NASH-related HCC patients identified the late neutrotime signature to be significantly enriched in NASH-HCC when compared with HCCs of other aetiologies44 (figure 6D). Moreover, the late neutrotime profile was specifically associated with human HCCs that are stratified by gene expression to the immune class and specifically within this group to the exhausted immune class which are typically resistant to immunotherapy (figure 6E).44–47 This suggests that TANs in human NASH-HCC resemble the mature phenotype of TANs in mouse NASH-HCC and may play a role in preventing ICI responses in patients, and as such we speculate they may be susceptible to similar therapeutic neutrotime reprogramming with AZD5069/anti-PD1 treatment. To examine the stage at which neutrophils are reprogrammed we compared intratumoural to circulating neutrophil profiles in the treatment groups in the DEN/ALIOS model. Neutrotime reprogramming was specific to the intratumoural population of AZD5069/anti-PD1 treated mice and noteably without an associated neutrotime change in circulating neutrophils of this treatment group (figure 6F), this observation being consistent with tumour-selective neutrophil reprogramming. Hence, while the combination therapy brings about reprogramming of TAN maturity, it leaves intact the mature phenotype of circulating neutrophils required for their classic anti-microbial surveillance functions.48 49
RNA-Seq of purified Ly6G+ neutrophils revealed that TANs from AZD5069/anti-PD1 treatment mice were enriched for process networks associated with cell cycle, phagocytosis and antigen presentation when compared with vehicle controls (figure 6G and online supplemental figure 7C). AZD5069 monotherapy modestly enhanced the expression of signatures associated with cell division, phagocytosis, and degranulation while also eliciting a reduction in protumour gene expression, with all of these effects being accentuated when AZD5069 was combined with anti-PD1 (figure 6G and online supplemental figure 7C–E). Anti-PD1 treatment promoted antigen presentation and processing signatures, which were also enriched in combined AZD5069/anti-PD1 treatment but not with AZD5069 monotherapy (figure 6G). These findings were again indicative of the combinatorial effects of AZD5069/anti-PD1 therapy on TAN phenotype. AZD5069 monotherapy (but not anti-PD1 monotherapy) suppressed the expression of key immune checkpoint molecules in TANs, including downregulation of Cd80, Pvr, Sirpa, Pdl1 and Pdl2. This loss of immune checkpoint gene expression was maintained in the context of combination therapy and for some genes (eg, Pvr and Srpa) we noted more pronounced suppressive effects when compared with the AZD5069 montherapy alone (online supplemental figure 7F). Hence, TAN-enriched immune hubs observed in AZD5069/anti-PD1 treated tumours are able to avoid ICI signals that might otherwise cause immune exhaustion. AZD5069/anti-PD1 TANs also displayed a strong correlation with transcriptional changes seen in neutrophils during an acute systemic inflammatory response,50 including expression of genes involved in exocytosis, myeloid cell activation and degranulation (online supplemental figure 7G,H). Finally, these AZD5069/anti-PD1 TANs closely resembled a recently objectively characterised acute-inflammatory immature-Ly6GInt neutrophil population isolated from lipopolysaccharide-(LPS)-treated mice50 (online supplemental figure 7I). In summary, AZD5069/anti-PD1 combination therapy brings about reprogramming of HCC-NASH TANs to exhibit immature, proliferative and inflammatory characteristics.
From these data we hypothesised that activated early neutrotime TANs have anti-tumoural properties. Due to their relatively low numbers and lack of specific surface markers it was not possible to isolate reprogrammed TANs from tumours in order to formally test this hypothesis. Instead, as proof-of-principle, we isolated inflammatory immature neutrophils enriched in the BM of LPS-treated mice and a pool of mature BM neutrophils isolated from control PBS treated mice. Adoptively transferring these cells to orthotopic NASH-HCC mice, we asked whether they would bring about an anti-tumoural effect in combination with anti-PD1 treatment (figure 6H and online supplemental figure 7J,K). Transfer of inflammatory immature neutrophils lead to a significant increase in circulating immature CXCR2Lo neutrophils in the blood and resulted in a significant reduction in tumour burden (figure 6I and online supplemental figure 7L). In contrast transfer of mature neutrophils had no effect on tumour burden (figure 6I). To investigate underlying mechanism we examined intratumoural cDC1 and CD8+ T cells. Similar to treatment of mice with AZD5069/anti-PD1, we noted transfused immature neutrophils caused increased activation (CD86+) of intratumoural XCR1+ cDC1 cells and elevated CD8+ T cells in tumours, unlike mice transfused with equal numbers of mature neutrophils (figure 6J–L). Moreover, the adoptive transfer of neutrophils from LPS treated was associated with increased intratumoural Gzmb expression indicative of stimulation of cytotoxic activity within the tumour (figure 6M). Hence, we conclude that BM derived immature inflammatory neutrophils which have phenotypic similarities to AZD5069/anti-PD1 reprogrammed TANs are able to stimulate immune remodelling within HCC tumours and promote anti-tumoural effects.
Discussion
Immune-based therapies hold considerable promise for the treatment of advanced HCC, however at present response rates are low and according to recent reports this is at least in-part determined by the immune cell composition of the tumour.45 51 52 HCC on the background of NASH presents additional considerations because of the crosstalk occurring between inflammatory cells and various metabolic adaptions manifest in the disease such as insulin resistance, steatosis, oxidative stress and altered mitochondrial function.53 Pfister and colleagues have reported that immunotherapy in NASH-HCC may be compromised due to high numbers of protumour CD8+PD1+ T cells in the tumour microenvironment.9 Here we show that selective targeting of neutrophils with a CXCR2 antagonist promotes the anti-tumour effects of anti-PD1 therapy in NASH-HCC, this effect being mechanistically associated with activation of classic CD8+ T cell and DC mediated anti-tumour immunity, but also with intratumoural reprogramming of TAN maturation and phenotype. Based on IMC we propose that the reprogrammed TANs, which are characterised by their proliferative and inflammatory characteristics, associate in tight clusters with CD8+ T cells and APCs to form anti-tumour Gzmb-secreting immune hubs within the NASH-HCC tumour microenvironment. Our work therefore emphasises the strong potential for targeted therapeutic manipulation of the innate immune system in cancer, but also uncovers a previously unrecognised crosstalk between the C-X-C chemokine/CXCR2 and PD1/PDL1 signalling systems that may be exploited to improve immunotherapy responses not only in NASH-HCC but also in other types of cancer that exhibit immunotherapy resistance.54 55
Neutrophil infiltration is a key pathological feature of human NASH that may result from upregulation of hepatic CXCL8 (IL-8) and CXCL1,56 57 which we also report here to be enriched in human NASH-HCC. In addition, expression of CXCR2 on neutrophils in NASH is selectively enhanced through an auto-stimulation mechanism involving the upregulation of neutrophil-derived lipocalin 2.58 Once present in the NASH and NASH-HCC microenvironments neutrophils are exposed to high levels of TGF-β which, as reported with other cancers,19–21 can polarise TANs towards a so-called ‘N2’ tumour-promoting state.14 It is also pertinent to address the relationship between TANs and myeloid-derived suppressor cells (MDSC), the latter being a heterogeneous population comprising polymorphonuclear granulocytic Ly6G+Ly6CLo (PMN-MDSC) and monocytic Ly6G-Ly6CHi (M-MDSC) cells. Accumulating evidence suggests that PMN-MDSC are immunosuppressive neutrophils and may be functionally very similar to the TANs that have been termed ‘N2’, with shared protumour properties.14 59 In the mouse there are no markers to distinguish between PMN-MDSCs and neutrophils and as such we cannot rule out that TANs in mouse models of NASH-HCC include PMN-MDSCs which may also be susceptible to reprogramming in response to combined CXCR2 antagonism and anti-PD1 therapy. However, the typical inhibitory effects on DC and CD8+ T cell functions associated with the activities of PMN-MDSCs and immunosuppressive neutrophils were clearly overcome by combined AZD5069/anti-PD1 therapy.
A growing body of evidence suggests that CXCR2 inhibition may be therapeutically beneficial in many human cancers including; pancreatic, lung, ovarian, prostate, colon and now the liver.26–30 60 Furthermore, in genetic murine models of lung cancer, inhibition of CXCR1 and 2 receptors in combination with anti-PD1 amplified anti-tumour responses.61 62 The proposed mechanism of action, until now, however, was thought to rely on reprogramming of the tumour immune microenvironment, primarily as a result of impaired myeloid recruitment. The most remarkable immunobiological finding of our study was that, paradoxically, when combined with anti-PD1, CXCR2 inhibition leads to an increase in tumour neutrophils and a selective reprogramming of the TAN neutrotime, with no evidence for a similar systemic effect on circulating neutrophils. The immature proliferative phenotype of the reprogrammed TANs evokes extramedullary granulopoiesis which can be seen in mice following antibody-mediated depletion of Ly6G+ cells and that is due to survival and expansion of residual tissue neutrophils driven by high systemic levels of granulocyte colony-stimulating factor,63 indeed this rebound effect meant that we were unable to exploit this protocol to directly interrogate the function of reprogrammed TANs. However, as proof-of-principle we were able to establish that adoptive transfer of immature activated neutrophils isolated from BM of LPS-treated mice has antitumour activity in NASH-HCC and this effect was accompanied by remodelling of tumour immunity including the activation of cDC1 cells, elevated CD8+ T cell counts and induction of anti-tumoural Gzmb; these being changes that were also noted with AZD506/anti-PD1 therapy. In future work it will be important to identify selective markers of the reprogrammed TANs that might be exploited for detailed functional characterisation, as well as for enabling their selective experimental manipulation which at present is not possible. Also, it will be important to determine precisely how and why combined CXCR2 antagonism and anti-PD1 treatment selectively induces proliferative immature neutrophils in the tumour. Clinically the ability to selectively reprogramme TANs while retaining mature anti-microbial neutrophils in the circulation may be very relevant in HCC since bacterial infections and septic shock are common clinical challenges in cirrhotic patients (in whom 90% of HCC develops).64
In summary, we present a novel combination immunotherapy that enhances the efficacy of anti-PD1 in NASH-HCC. As the CXCR2 antagonist AZD5069 has been demonstrated to be safe for use in humans it is timely to determine if HCC patients would benefit from a similar therapy.
Methods
Mice ethical approval
All animal experiments using the orthotopic NASH-HCC model and DEN/ALIOS model were performed in accordance with a UK Home Office licence (PP8854860, PP390857 and PP0604995), adhered to ARRIVE guidelines (https://www.nc3rs.org.uk/arrive-guidelines), and in accordance with the UK Animal (Scientific Procedures) Act 1986, and were subject to review by the animal welfare and ethical review board of the University of Glasgow and Newcastle University. All mice were housed in specific pathogen free conditions with unrestricted access to food and water and maintained on a constant 12 hours light-dark cycle under controlled climate (19°C–22°C, 45%–65% humidity). All animal experiments using the CD-HFD were performed in accordance with German law and the governmental bodies, and with approval from the Regierungspräsidium Karlsruhe (G11/16, G129/16, G7/17). Male mice were housed at the German Cancer Research Centre (DKFZ) (constant temperature of 20°C–24°C and 45%–65% humidity with a 12 hours light-dark cycle and were maintained under specific pathogen-free conditions.
Quantification and statistical analysis
Statistical analyses were performed using GraphPad Prism software (V.9 GraphPad Software, La Jolla, CA, USA) and R (V.3.5.1) performing tests as indicated and were considered statistically significant. P values are included in figures.
Additional methods are described in online supplemental materials.
Supplemental material
Supplemental material
Data availability statement
Data are available in a public, open access repository. All data will be deposited with accession codes, unique identifiers or web links for publicly available datasets provided before publication.
Ethics statements
Patient consent for publication
Ethics approval
Collection and use of human tissue were ethically approved by the North East – Newcastle and North Tyneside 1 Research Ethics Committee. Human liver tissue from surgical resections was obtained under full ethical approval (H10/H0906/41) and through the CEPA biobank (17/NE/0070) and used subject to patients written consent. HCC tumour and non-tumour biopsy tissue was obtained under full ethical approval as approved by the Newcastle and North Tyneside Regional Ethics Committee, the Newcastle Academic Health Partners Bioresource (NAHPB) and the Newcastle upon Tyne NHS Foundation Trust Research and Development (R&D) department. (Reference numbers: 10/H0906/41; NAHPB Project 48; REC 12/NE/0395; R&D 6579; Human Tissue Act licence 12534).
Acknowledgments
We would like to that the core services and advanced technologies at the CRUK Beatson Institute with particular thanks to the Biological Services Unit, Molecular Services, Bioinformatics, Histology Department and the Beatson Advanced Imaging Resource. We would like to thank Danijela Heide, Jenny Hetzer for technical support for the CD-HFD NASH-HCC model. We would like to thank Catherine Winchester and Nathalie Sphyris for critical reading of the manuscript. We would like to thank the Newcastle University Comparative Biology Centre, Newcastle University Bioimaging Unit and the Newcastle University Flow cytometry core facility for technical assistance.
References
Supplementary materials
Supplementary Data
This web only file has been produced by the BMJ Publishing Group from an electronic file supplied by the author(s) and has not been edited for content.
Supplementary Data
This web only file has been produced by the BMJ Publishing Group from an electronic file supplied by the author(s) and has not been edited for content.
Footnotes
JL, JBGM and TJ are joint first authors.
JML, LMC, TGB, OJS and DAM are joint senior authors.
Twitter @FFERCOQ, @ef_roger, @DrCEWilloughby, @mimue_lab
Correction notice This article has been corrected since it published Online First. The joint senior shared author statement has been added and the corresponding author's address updated.
Contributors JL, JM and TJ performed the majority of the laboratory-based work and analyses presented in the manuscript. ER, TD, FF, WC, KG, AH, CN, SL, ML, RP, PH, RE, CEW, MR, CAF, DP, SR, NW, MVM, AC, DG, AF, DM, AF, XC-L, N-EM, CAF, XLRI, AJM, MVM and RAR performed a portion of the laboratory experiments and their related analyses. ER, SB, JML, MFH and GG provided advice and/or contributed to the experimental design and writing. JL, JM, HR, LC, TB, OJS and DAM conceived the studies, designed the experiments and wrote the manuscript. All authors read and commented on the final manuscript. DAM, OJS, HR, LC and TB provided funding. DAM acts as guarantor for the study.
Funding DM, OJS, HR and TB were supported by program grant funding from CRUK (C9380/A26813). DM was supported by MRC program Grants MR/K0019494/1 and MR/R023026/1. DM, OJS, HR, TB, JM and JML are supported by a CRUK programme grant (C18342/A23390). OJS is funded by a CRUK grant (CRUK A21339). LC is funded by a CRUK grant (CRUK A23983). TB receives research funding support from AstraZeneca. TB and MM were funded by the Wellcome Trust (WT107492Z). HR was funded by CRUK Newcastle Experimental Cancer Medicine Centre award (C9380/A18084). JM and TJ were supported by CRUK core funding (A17196 and A31287). JL was supported by funding from the Faculty of Medical Sciences, Newcatle University. DG is supported by the Newcastle CRUK Clinical Academic Training Programme. AC is funded by the WE Harker Foundation. RE is supported by a doctoral training grant from MICINN/MINECO (BES-2017-081286) and a mobility grant from Fundació Universitària Agustí Pedro i Pons. CEW is supported by a Sara Borrell fellowship (CD19/00109) from the Instituto de Salud Carlos III (ISCIII) and the European Social Fund. PH is supported by a fellowship grant from the German Research Foundation (DFG, HA 8754/1-1). CA-O is supported by a predoctoral research scholarship from Fulbright España. JL is supported by grants from the NIH (RO1DK56621 and RO1DK128289), the Samuel Waxman Cancer Research Foundation, the Spanish National Health Institute (PID2019-105378RB-I00), through an Accelerator award in partnership between Cancer Research UK, Fondazione AIRC and Fundación Científica de la Asociación Española Contra el Cáncer (HUNTER, C9380/A26813), and by the Generalitat de Catalunya (AGAUR, SGR-1358).
Competing interests DM is a director of Fibrofind. JL and DM are shareholders in Fibrofind limited. SB owns shares in AstraZeneca. OJS receives funding from AstraZeneca and Novartis. TGB receives research funding support from AstraZeneca. JML receives research support from Bayer HealthCare Pharmaceuticals, Eisai Inc, Bristol-Myers Squibb, Boehringer-Ingelheim and Ipsen, and consulting fees from Eli Lilly, Bayer HealthCare Pharmaceuticals, Bristol-Myers Squibb, Eisai Inc, Celsion Corporation, Exelixis, Merck, Ipsen, Genentech, Roche, Glycotest, Nucleix, Sirtex, Mina Alpha and AstraZeneca.
Patient and public involvement Patients and/or the public were not involved in the design, or conduct, or reporting, or dissemination plans of this research.
Provenance and peer review Not commissioned; externally peer reviewed.
Supplemental material This content has been supplied by the author(s). It has not been vetted by BMJ Publishing Group Limited (BMJ) and may not have been peer-reviewed. Any opinions or recommendations discussed are solely those of the author(s) and are not endorsed by BMJ. BMJ disclaims all liability and responsibility arising from any reliance placed on the content. Where the content includes any translated material, BMJ does not warrant the accuracy and reliability of the translations (including but not limited to local regulations, clinical guidelines, terminology, drug names and drug dosages), and is not responsible for any error and/or omissions arising from translation and adaptation or otherwise.