OBJECTIVE: The aim of this study was to evaluate the relationship between cytokine production, GM-CSF receptor (CSF2RA), and IL-1 receptor (IL1R2) expression in mammary adenocarcinoma and their association with it histopathological parameters and lymph node metastasis. METHODS: We analyzed tumor biopsy samples (cultured in vitro) from 50 women (aged 43-75) with invasive ductal mammary adenocarcinomas. Enzyme-linked immunosorbent assay method the concentrations of interleukin 2, interleukin 6, interleukin 8, interleukin 10, interleukin 17, interleukin 18, interleukin 1β, interleukin 1Ra, tumor necrosis factor α, interferon γ, granulocyte colony-stimulating factor, granulocyte macrophage colony-stimulating factor, and vascular endothelial growth factor A were determined in culture supernatants. The expression of CSF2RA and IL1R2 in tumor biopsy was evaluated by immunohistochemical method. RESULTS: We showed that the "cytokine profile" of a tumor (the ability of tumor cells and its microenvironment to produce different cytokines) is very individual. It has been shown that the features of the cytokine profile of the mammary adenocarcinoma are important for the formation and realization of the metastatic potential of the mammary adenocarcinoma. We found correlations between some histopathological parameters of mammary adenocarcinoma and coefficients KGM-CSF/CSF2RA and KIL-1β/IL1R2, which are the ratios of concentrations of granulocyte macrophage colony-stimulating factor and interleukin -1β to expression of CSF2RA and IL1R2, respectively. KGM-CSF/CSF2RA positively correlated with highly differentiated cells, and KIL-1β/IL1R2 positively correlated with the number of mitoses, poorly differentiated cells, and a number of lymph nodes with metastases. KGM-CSF/CSF2RA positively correlated with the concentrations of interleukin 6, interleukin 8, interleukin 1Ra, and granulocyte colony-stimulating factor. KIL-1β/IL1R2 positively correlated with concentrations of interleukin 1β and interferon γ and negative correlated with the concentrations of vascular endothelial growth factor A and tumor necrosis factor α. It is shown that KIL-1β/IL1R2 can be considered as a prognostic indicator predicting the probability of mammary adenocarcinoma metastasis to regional lymph nodes. CONCLUSIONS: The ratios of granulocyte macrophage colony-stimulating factor and interleukin 1β cytokines, produced in tumor, to the expression of CSF2RA and IL1R2 depend on levels of interleukin 6, interleukin 8, tumor necrosis factor α, interferon γ, granulocyte colony-stimulating factor, and vascular endothelial growth factor A and are important factors affecting the progression and metastasis of the breast cancer.
OBJECTIVE: The aim of this study was to evaluate the relationship between cytokine production, GM-CSF receptor (CSF2RA), and IL-1 receptor (IL1R2) expression in mammary adenocarcinoma and their association with it histopathological parameters and lymph node metastasis. METHODS: We analyzed tumor biopsy samples (cultured in vitro) from 50 women (aged 43-75) with invasive ductal mammary adenocarcinomas. Enzyme-linked immunosorbent assay method the concentrations of interleukin 2, interleukin 6, interleukin 8, interleukin 10, interleukin 17, interleukin 18, interleukin 1β, interleukin 1Ra, tumor necrosis factor α, interferon γ, granulocyte colony-stimulating factor, granulocyte macrophage colony-stimulating factor, and vascular endothelial growth factor A were determined in culture supernatants. The expression of CSF2RA and IL1R2 in tumor biopsy was evaluated by immunohistochemical method. RESULTS: We showed that the "cytokine profile" of a tumor (the ability of tumor cells and its microenvironment to produce different cytokines) is very individual. It has been shown that the features of the cytokine profile of the mammary adenocarcinoma are important for the formation and realization of the metastatic potential of the mammary adenocarcinoma. We found correlations between some histopathological parameters of mammary adenocarcinoma and coefficients KGM-CSF/CSF2RA and KIL-1β/IL1R2, which are the ratios of concentrations of granulocyte macrophage colony-stimulating factor and interleukin -1β to expression of CSF2RA and IL1R2, respectively. KGM-CSF/CSF2RA positively correlated with highly differentiated cells, and KIL-1β/IL1R2 positively correlated with the number of mitoses, poorly differentiated cells, and a number of lymph nodes with metastases. KGM-CSF/CSF2RA positively correlated with the concentrations of interleukin 6, interleukin 8, interleukin 1Ra, and granulocyte colony-stimulating factor. KIL-1β/IL1R2 positively correlated with concentrations of interleukin 1β and interferon γ and negative correlated with the concentrations of vascular endothelial growth factor A and tumor necrosis factor α. It is shown that KIL-1β/IL1R2 can be considered as a prognostic indicator predicting the probability of mammary adenocarcinoma metastasis to regional lymph nodes. CONCLUSIONS: The ratios of granulocyte macrophage colony-stimulating factor and interleukin 1β cytokines, produced in tumor, to the expression of CSF2RA and IL1R2 depend on levels of interleukin 6, interleukin 8, tumor necrosis factor α, interferon γ, granulocyte colony-stimulating factor, and vascular endothelial growth factor A and are important factors affecting the progression and metastasis of the breast cancer.
To date, multiple research articles have been published showing that cytokines should be
considered an important factor affecting pathological mechanisms of malignant tumor
formation, progression, and metastases.[1,2] During tumor growth, cytokines are produced not only in immune organs and in the
immunocompetent cells that infiltrate the tumor but also directly by the tumor cells
together with the cells of the connective tissue that form the microenvironment of the tumor.[3,4] Moreover, the cytokine network that develops in the tumor becomes one of the most
important regulators of cell–cell interaction within the tumor.[5,6]Several studies have shown that depending on the concentration and balance of the levels of
cytokines and their antagonists, they can enhance or inhibit breast cancer growth and metastases.[7,8] For example, changes in the relative concentration of some cytokines (interleukin
[IL]-1, IL-6, IL-8, IL-11, IL-18, and IL-19) and growth factors (granulocyte
colony-stimulating factor [G-CSF], granulocyte macrophage colony-stimulating factor
[GM-CSF], and vascular endothelial growth factor A [VEGF-A]) in blood can directly or
indirectly stimulate breast cancer growth or progression.[9,10] However, the mechanisms of this effect have not been studied enough, since most of
the data on the role of cytokines in tumor progression are based, as a rule, only on the
comparison of data on the concentration of certain cytokines detected in the blood with
tumor growth rates.Recently, in our laboratory, it was shown that mammary adenocarcinoma (MAC) biopsy samples,
obtained from tumors metastasizing to regional lymph nodes, produced in tissue culture
in vitro significantly more GM-CSF and IL-1β cytokines than bioptates of
nonmetastatic breast tumors.[11] We have also shown that that the high-level production of IL-1β and IL-18 by MAC,
overexpression of VEGF-R2 in tumor (at relatively low VEGF-A production), and the high level
of interferon γ (IFN-γ) production are attributed factors contributing to the formation of a
population of low-grade cells in the tumor.[12] In this regard, from a theoretical and practical point of view, it was interesting to
study the possibility of using the same model to evaluate the production of some cytokines
produced by the tumor as well as some receptors for cytokines expressed in tumor cells, in
relation to histopathological parameters of the tumor, as prognostic biological markers
indicating the probability of MAC metastasis to regional lymph nodes.The aim of our research to study the relationship between cytokine production, CSF2RA, and
IL1R2 expression in MAC and their association with it histopathological parameters and lymph
node metastasis.
Materials and Methods
Patients
The object of the study was cultured tumor biopsy samples from 50 women aged 43 to 75
with invasive ductal breast cancer (according to modern classification revised World
Health Organization in 2012—“Invasive Breast Carcinoma of No Special Type” [NST]), treated
at the Novosibirsk Regional Oncological Center, which was classified according to
histological type as MAC grade II to III. The exclusion criteria from the study were signs
of hematogenous metastasis to distant organs and the presence of concomitant hormonal,
chronic, inflammatory, and infectious diseases. The study and all study protocols have
been approved by the Ethics Committee of the Institute of Molecular Biology and Biophysics
(Approval No. 2016-3) and Subdivision of Federal Research Center of Fundamental and
Translational Medicine (Novosibirsk, Russia). All procedures performed in this study were
conducted in accordance with the 1964 Helsinki Declaration and its later amendments or
comparable ethical standards. Each patient was informed about the study conducted and its
objectives and methods. Written informed consent for participation in the study and for
the tumor biopsy procedure was signed by each patient and verified by a physician.
Method of Measurement of Cytokine Production
Tumor biopsy samples (8 mm3), obtained using core biopsy,[11] were washed with culture medium Dulbecco modified Eagle medium (DMEM)–F12 3 times
to wash off the remaining blood cells on their surface and then were placed into a glass
vial with 1 mL of the DMEM–F12 growth medium and incubated for 72 hours in order to
accumulate in the supernatant sufficient (for an accurate assessment of each cytokine)
concentration of all the cytokines studied by us. Before collection of the supernatant,
the tumor biopsy samples were retrieved from the vial and placed in 10% neutral formalin.
After culturing the biopsy samples in the supernatant, there was a small number (no more
than 50-100 cells for the whole supernatant) of cellular elements (single tumor, lymphoid,
and monocytic cells) that were removed from supernatant by precipitating with
centrifugation at 900 × g for 15 minutes. By enzyme-linked immunosorbent
assays (the assay kits produced by AO Vector-Best (Novosibirsk Region, Russia)), the
concentrations of IL-2, IL-6, IL-8, IL-10, IL-17, IL-18, IL-1β, IL-1Ra, tumor necrosis
factor α (TNF-α), IFN-γ, G-CSF, GM-CSF, and VEGF-A were determined in the culture
supernatant.
Immunohistochemical Analysis
The MAC biopsy samples fixed in neutral formalin were dehydrated and embedded in
paraffin. Dewaxing and rehydration of the MAC paraffin sections were carried out according
to the standard procedure through xylene and alcohol. The expression of CSF2RA and IL1R2
receptors was evaluated in 2 tumor samples of each patient obtained simultaneously. One
sample was examined immediately, and the second after 72 hours of cultivation. The
expression of CSF2RA and IL1R2 in MAC sections was detected using antibodies of
appropriate specificity (anti-CSF2RA, MBS711361; MyBioSource [San Diego, California, USA];
anti-IL1R2, LS-B377, LifeSpan [Seattle, Washington, USA]), and visualization system
VECTASTAIN Elite ABC Kit (Vector Laboratories [Burlingame, California, USA], PK-7200)
according to the manufacturer’s recommendations. The slices were additionally stained with
Azure II–eosin, dehydrated, and embedded in balsam.
Computer Morphometric Analysis
Histological samples stained for CSF2RA and IL1R2 were photographed (at magnification
400×) using an image analysis system based on a Micros MC 300A microscope (Austria) and a
digital CMOS camera based on the Aptina MT9J003 sensor (China). Computer morphometric
quantitative evaluation of expression of receptors CSF2RA and IL1R2 was performed in the
ImageJ 1.50a software (National Institute of Health, Bethesda, Maryland).
Immunohistochemical indicators of CSF2RA and IL1R2 expression were as squares of colored
zones that were specific for CSF2RA and IL1R2 expression (%, percentage of colored area
from a total area of tested image, based on 8 digital photographs).
KGM-CSF/CSF2RA and KIL-1β/IL1R2 coefficients were then determined,
representing the ratio of the concentration of cytokines GM-CSF and IL-1β to expression
value of CSF2RA and IL1R2 receptors, respectively. The coefficients are expressed in
arbitrary units.
Histopathological Analysis
After surgical resection, a pathologist carried out a histopathological examination of
the MAC tissue sections stained with hematoxylin and eosin according to the standard
procedure. Evaluation of the differentiation degree of the tumor cells and their
classification as highly differentiated, moderately differentiated, and poorly
differentiated cells were based on the cellular polymorphism degree, nuclear–cytoplasmic
ratio, presence of mitoses (including pathological ones), capacity for tissue structure
formation (gland development), and preservation of cell functions.[13,14] Highly differentiated tumor cells had a shape similar to that of normal cells and
showed the predominance of cytoplasm over nucleus and capacity for gland formation. Poorly
differentiated tumor cells had an irregular shape and featured pronounced polymorphism,
predominance of the nucleus over cytoplasm, inability to form tissue structures, diffuse
growth, and numerous mitoses (including pathological ones). Moderately differentiated
tumor cells were somewhere between and in terms of these features. We calculated the mean
number of mitoses and pathological mitoses after analyzing 10 visual fields as well as the
percentage of poorly differentiated, moderately differentiated, and highly differentiated
tumor cells.
Statistical Analysis
Histograms was created in the Microsoft Excel, Statistica version 7, and IBM SPSS
Statistics version 22.0. Determination of mean values, medians, 25th to 75th percentiles,
and Spearman rank correlation coefficient (r) was performed by means of
software package Statistica version 7. The cluster analysis was performed using the
Statistica version 7. Receiver operating characteristic (ROC) curve analysis was performed
by means of software package IBM SPSS Statistics version 22.0.
Results
Cytokine Profiles of the Supernatants of MAC Samples
At the beginning of the study, we examined individual cytokine profiles in MAC samples of
different patients. The concentrations of IL-2, IL-6, IL-8, IL-10, IL-17, IL-18, IL-1β,
IL-1Ra, TNF-α, IFN-γ, G-CSF, GM-CSF, and VEGF-A were determined in the culture
supernatants. The cytokine profiles of MAC samples obtained from different patients
differed considerably (Figure 1).
This difference manifested itself in considerable variation in concentrations of some
cytokines in MAC culture supernatants and, accordingly, different proportions of cytokines
in the resulting individual profile of each patient. The generalized estimation of the
levels of production of cytokines (medians, 25th and 75th percentiles) is shown in Figure 2. The greatest variability in
values was revealed for the following cytokines produced by MAC samples (in ascending
order): GM-CSF, IL-1β, IL-8, IL-6, and IL-18.
Figure 1.
Cytokine profiles in the supernatants of mammary adenocarcinoma (MAC) biopsy samples
that were obtained from 50 patients (cumulative histograms): interleukin (IL)-2,
IL-10, IL-17, IL-18, IL-1β, tumor necrosis factor α (TNF-α), interferon γ (IFN-γ),
granulocyte macrophage colony-stimulating factor (GM-CSF), IL-6, IL-8, IL-1Ra,
granulocyte colony-stimulating factor (G-CSF), and vascular endothelial growth factor
A (VEGF-A). Tumor samples (8 mm3), obtained using core biopsy, were placed
into a sterile vial with 1 mL of the Dulbecco modified Eagle medium (DMEM)–F12 growth
medium for 72 hours. By means of a solid-phase immunosorbent assay, the cytokine
concentrations were determined in the MAC supernatants (pg/mL).
Figure 2.
The value of concentrations (pg/mL) of interleukin (IL)-2, IL-6, IL-8, IL-10, IL-17,
IL-18, IL-1β, IL-1Ra, tumor necrosis factor α (TNF-α), interferon γ (IFN-γ),
granulocyte colony-stimulating factor (G-CSF), granulocyte macrophage
colony-stimulating factor (GM-CSF), and vascular endothelial growth factor A (VEGF-A)
in the supernatants of mammary adenocarcinoma (MAC) biopsy samples that were obtained
from 50 patients. Tumor samples (8 mm3), obtained using core biopsy, were
placed into a sterile vial with 1 mL of the Dulbecco modified Eagle medium (DMEM)–F12
growth medium for 72 hours. By means of a solid-phase immunosorbent assay, the
cytokine concentrations were determined in the MAC supernatants. The data were
presented as median ± 25th to 75th percentiles.
Cytokine profiles in the supernatants of mammary adenocarcinoma (MAC) biopsy samples
that were obtained from 50 patients (cumulative histograms): interleukin (IL)-2,
IL-10, IL-17, IL-18, IL-1β, tumor necrosis factor α (TNF-α), interferon γ (IFN-γ),
granulocyte macrophage colony-stimulating factor (GM-CSF), IL-6, IL-8, IL-1Ra,
granulocyte colony-stimulating factor (G-CSF), and vascular endothelial growth factor
A (VEGF-A). Tumor samples (8 mm3), obtained using core biopsy, were placed
into a sterile vial with 1 mL of the Dulbecco modified Eagle medium (DMEM)–F12 growth
medium for 72 hours. By means of a solid-phase immunosorbent assay, the cytokine
concentrations were determined in the MAC supernatants (pg/mL).The value of concentrations (pg/mL) of interleukin (IL)-2, IL-6, IL-8, IL-10, IL-17,
IL-18, IL-1β, IL-1Ra, tumor necrosis factor α (TNF-α), interferon γ (IFN-γ),
granulocyte colony-stimulating factor (G-CSF), granulocyte macrophage
colony-stimulating factor (GM-CSF), and vascular endothelial growth factor A (VEGF-A)
in the supernatants of mammary adenocarcinoma (MAC) biopsy samples that were obtained
from 50 patients. Tumor samples (8 mm3), obtained using core biopsy, were
placed into a sterile vial with 1 mL of the Dulbecco modified Eagle medium (DMEM)–F12
growth medium for 72 hours. By means of a solid-phase immunosorbent assay, the
cytokine concentrations were determined in the MAC supernatants. The data were
presented as median ± 25th to 75th percentiles.
Evaluation of the Variability in Cytokine Profiles of MAC Biopsy Samples by Cluster
Analysis
To assess the variability in cytokine profiles of MAC biopsy samples, we used
hierarchical cluster analysis, which allows us to classify the objects of study by a large
number of parameters.In our study, we used as such parameters the production of 13 cytokines produced by MAC
biopsy samples in vitro (concentration of cytokines in the supernatant,
pg/mL). Using Ward’s cluster method, it was found that with Linkage distance within 13 to
18, all cytokine profiles can be divided into 3 clusters and, accordingly, into 3 groups
of profiles of cytokine production in MAC (Figure 3). It is important to note that cluster 2
received a large number of cytokine profiles of those MAC samples that were obtained from
patients with metastases to the lymph nodes. Cluster 2 contained indicators of cytokine
production in 66.7% of patients with metastases in regional lymph nodes, relative to the
total number of patients who had metastases.
Figure 3.
Hierarchical dendrogram obtained by clustering mammary adenocarcinoma (MAC) biopsies
of 50 patients by concentrations of 13 cytokines produced by MAC biopsies. Ward’s
cluster method. Cluster 1 and cluster 3 contained indicators of cytokine production in
equal numbers—about 16.7% of patients with metastases to regional lymph nodes,
relative to the total number of patients who had metastases. Cluster 2 contained
indicators of cytokine production in 66.7% of patients with metastases in regional
lymph nodes, relative to the total number of patients who had metastases.
Hierarchical dendrogram obtained by clustering mammary adenocarcinoma (MAC) biopsies
of 50 patients by concentrations of 13 cytokines produced by MAC biopsies. Ward’s
cluster method. Cluster 1 and cluster 3 contained indicators of cytokine production in
equal numbers—about 16.7% of patients with metastases to regional lymph nodes,
relative to the total number of patients who had metastases. Cluster 2 contained
indicators of cytokine production in 66.7% of patients with metastases in regional
lymph nodes, relative to the total number of patients who had metastases.Cluster 1 and cluster 3 contained indicators of cytokine production in equal
numbers—about 16.7% of patients with metastases to regional lymph nodes, relative to the
total number of patients who had metastases.The data obtained indicated that the features of the cytokine profile of the MAC are
important for the formation and realization of the metastatic potential of the MAC.
Peculiarities of Expression of CSF2RA and IL1R2 in the Samples of MAC and the Ratios
of Concentrations of GM-CSF and IL-1β to Expression of CSF2RA and IL1R2,
Respectively
In the study of tumor samples after cultivation for 72 hours, it was noted that the
morphological structure did not differ from the samples of the same tumor before
cultivation. They were characterized by a typical structure with the formation of nests,
clusters, and trabeculae. No signs of redistribution of cell elements of lymphocytic and
macrophage type due to migration, which could be caused by the process of cultivation in
the samples, were identified. The average value of CSF2RA expression (colored area to
total area of tested image, %; mean ± standard error) in MAC samples without cultivation
was—2.11 ± 0.32, and in samples after cultivation 72 hours—1.74 ± 0.35 (P
> .05). The average value of IL 1R2 expression in MAC samples without cultivation was
4.15 ± 0.59, and in samples after cultivation 72 hours was 3.79 ± 0.65 (P
> .05). For further study and calculation, KGM-CSF/CSF2RA and
KIL-1β/IL1R2 coefficients used the data on the expression of IL1R2 and
CSF2RA, expressed in samples of MAC after cultivation for 72 hours, because from these
samples were obtained supernatants in which were determined the concentrations of various
cytokines.Figure 4A and B presents data on
the distribution of data by the following indicators: percentage of CSF2RA-colored area
(to total area of tested image) as an indicator of CSF2RA expression and
KGM-CSF/CSF2RA coefficient representing the ratio of the concentration of
GM-CSF to expression value of CSF2RA. The least variability was determined for the
expression of CSF2RA.
Figure 4.
Histograms showing a distribution of data by the following indicators in mammary
adenocarcinoma (MAC) biopsy samples. A, Percentage of CSF2RA-colored area (to total
area of tested image) as an indicator of CSF2RA expression; (B)
KGM-CSF/CSF2RA coefficient representing the ratio of the concentration of
granulocyte macrophage colony-stimulating factor (GM-CSF; pg/mL) to expression value
of CSF2RA (percentage of CSF2RA specific colored area); (C) percentage of
IL1R2-colored area (to total area of tested image) as an indicator of IL1R2
expression; (D) KIL-1β/IL1R2 coefficient representing the ratio of the
concentration of interleukin (IL)-1β (pg/mL) to expression value of IL1R2 (percentage
of IL1R2 specifically colored area). The data were presented as median ± 25th to 75th
percentiles.
Histograms showing a distribution of data by the following indicators in mammary
adenocarcinoma (MAC) biopsy samples. A, Percentage of CSF2RA-colored area (to total
area of tested image) as an indicator of CSF2RA expression; (B)
KGM-CSF/CSF2RA coefficient representing the ratio of the concentration of
granulocyte macrophage colony-stimulating factor (GM-CSF; pg/mL) to expression value
of CSF2RA (percentage of CSF2RA specific colored area); (C) percentage of
IL1R2-colored area (to total area of tested image) as an indicator of IL1R2
expression; (D) KIL-1β/IL1R2 coefficient representing the ratio of the
concentration of interleukin (IL)-1β (pg/mL) to expression value of IL1R2 (percentage
of IL1R2 specifically colored area). The data were presented as median ± 25th to 75th
percentiles.The greatest variability was found for KGM-CSF/CSF2RA coefficient. The
histopathological and immunohistochemical analyses of MAC biopsy samples show that the
receptor CSF2RA in the samples was expressed predominantly in monocytes/macrophages of
infiltrating the tumor. Outlier and extreme CSF2RA expression values were due to the
presence of macrophage infiltrates expressing CSF2RA in some samples of MAC (Figure 4A). Figure 4C and D presents data on the distribution of
data on the following indicators: percentage of IL1R2-colored area (to total area of
tested image) as expression KIL-1β/IL1R2 coefficient representing the ratio of
the concentration of IL-1β to expression value of IL1R2. The smallest variability was
determined for the expression of IL1R2 (IL1R2 percentage of colored area). The greatest
variability was found for KIL-1β/IL1R2 coefficient (Figure 4D). The histopathological and
immunohistochemical analyses of MAC biopsy samples show that the receptor IL1R2 was
expressed predominantly in monocytes/macrophages. The outlier and extreme values of IL1R2
expression were due to the presence of tumor cells expressing IL1R2 in some of the MAC
samples (Figure 4C).
Correlation Between CSF2RA and IL1R2 Expression,
KGM-CSF/CSF2RA, and KIL-1
β/IL1R2 Coefficients With Histopathological Indicators and Metastasis Rate in
Regional Lymph Nodes
As for CSF2RA and IL1R2 expression correlations, we found a correlation only between
CSF2RA expression and the percentage of highly differentiated cells in MAC samples (a
positive correlation) and between IL1R2 expression and the proportion of highly
differentiated cells in MAC samples (a negative correlation; Table 1) and number of regional lymph nodes with
metastases (a positive correlation). More often, a correlation of coefficients
KGM-CSF/CSF2RA and KIL-1β/IL1R2 with histopathological parameters
(Table 1) was
identified.
Table 1.
Coefficients (r) of Correlation Between of CSF2RA and IL1R2
Expression, KGM-CSF/CSF2RA, and KIL-1β/IL1R2 With
Histopathological Parameters of MAC.
Coefficients (r) of Correlation Between of CSF2RA and IL1R2
Expression, KGM-CSF/CSF2RA, and KIL-1β/IL1R2 With
Histopathological Parameters of MAC.Abbreviations: GM-CSF, granulocyte macrophage colony-stimulating factor; MAC,
mammary adenocarcinoma.Table 1 indicates that
parameter KGM-CSF/CSF2RA negatively correlated with the percentage of
moderately differentiated cells (r = −.44) and positively correlated with
the percentage of highly differentiated cells (r = .59). Parameter
KIL-1β/IL1R2 showed a negative correlation with the percentage of highly
differentiated tumor cells in MAC (r = −.51) and number of lymph nodes
with metastases and a positive correlation with the histopathological parameters of MAC
that determine the grade of tumor malignancy: the numbers of mitoses (r =
.50) and pathological mitoses (r = .48) and the percentage of poorly
differentiated cells (r = .57).
Search and Evaluation of the Quality of ROC Models, Including
KGM-CSF/CSF2RA and KIL-1
β/IL1R2, to Explore the Possible Influence of the Interaction of CSF2RA and
IL1R2 With the Corresponding Cytokines on the Process of Metastasis MAC in Regional Lymph
Nodes
In order to evaluate the quality of models, including KGM-CSF/CSF2RA and
KIL-1β/IL1R2, to explore the possible influence of the interaction of CSF2RA
and IL1R2 with the corresponding cytokines on the process of metastasis MAC in regional
lymph nodes, we used the ROC analysis. The ROC curves allowed us to evaluate the quality
of the models by dividing all patients into the groups (or classes). In our model, such
groups include patients with metastases in regional lymph nodes and patients without
metastases in regional lymph nodes. Despite the lack of correlations between number of
lymph nodes with metastases and GM-CSF concentrations and KGM-CSF/CSF2RA (Table 1), using indicators GM-CSF
and KGM-CSF/CSF2RA of all patients, we obtained an average quality model (AUC =
0.625) for the division of patients into 2 groups—with metastases in the lymph nodes and
without metastases (Figure
5A).
Figure 5.
Receiver operating characteristic (ROC) curves, characterizing the quality of the ROC
models for dividing all patients with mammary adenocarcinoma (MAC) into 2
groups—patients with metastases to regional lymph nodes and patients without
metastases, by values granulocyte macrophage colony-stimulating factor (GM-CSF;
pg/mL), CSF2RA (colored area, %), and KGM-CSF/CSF2RA (conventional units;
A) for all patients: for GM-CSF area under the curve (AUC) = 0.633, for CSF2RA AUC =
0.573, for KGM-CSF/CSF2RA AUC = 0.625; (B) provided that highly
differentiated tumor cells in MAC biopsy specimens were in the range of 10% to 30% for
GM-CSF AUC = 0.692, for CSF2RA AUC = 0.514, for KGM-CSF/CSF2RA AUC = 0.653.
ROC curves, characterizing the quality of the ROC models by dividing the 2 groups of
patients—with metastases to regional lymph nodes and without metastases, by values (B)
IL-1β (pg/mL), IL1R2 (colored area, %), and KIL-1β/IL1R2 (conventional
units); (C) for all patients: for IL-1β AUC = 0.616, for IL1R2 AUC = 0.226,
KIL-1β/IL1R2 AUC = 0.770; (D) provided that highly differentiated tumor
cells in MAC biopsy specimens were in the range of 10% to 30%: for IL-1β AUC = 707.0,
for IL1R2 AUC = 0.093, for KIL-1β/IL1R2 AUC = 0.913.
Receiver operating characteristic (ROC) curves, characterizing the quality of the ROC
models for dividing all patients with mammary adenocarcinoma (MAC) into 2
groups—patients with metastases to regional lymph nodes and patients without
metastases, by values granulocyte macrophage colony-stimulating factor (GM-CSF;
pg/mL), CSF2RA (colored area, %), and KGM-CSF/CSF2RA (conventional units;
A) for all patients: for GM-CSF area under the curve (AUC) = 0.633, for CSF2RA AUC =
0.573, for KGM-CSF/CSF2RA AUC = 0.625; (B) provided that highly
differentiated tumor cells in MAC biopsy specimens were in the range of 10% to 30% for
GM-CSF AUC = 0.692, for CSF2RA AUC = 0.514, for KGM-CSF/CSF2RA AUC = 0.653.
ROC curves, characterizing the quality of the ROC models by dividing the 2 groups of
patients—with metastases to regional lymph nodes and without metastases, by values (B)
IL-1β (pg/mL), IL1R2 (colored area, %), and KIL-1β/IL1R2 (conventional
units); (C) for all patients: for IL-1β AUC = 0.616, for IL1R2 AUC = 0.226,
KIL-1β/IL1R2 AUC = 0.770; (D) provided that highly differentiated tumor
cells in MAC biopsy specimens were in the range of 10% to 30%: for IL-1β AUC = 707.0,
for IL1R2 AUC = 0.093, for KIL-1β/IL1R2 AUC = 0.913.The AUC values for GM-CSF (pg/mL), CSF2RA (colored area, %), and
KGM-CSF/CSF2RA (conventional units) were, respectively, 0.633, 0.573, and
0.625. The quality of the ROC model for the division of the patient group into a subgroup
of patients without lymph node metastases and, accordingly, into a subgroup of patients
with metastases, based on the use of indicators GM-CSF and KGM-CSF/CSF
2RA, practically did not change when taking into account the indicators of only
those patients (n = 31), in which the relative content of highly differentiated tumor
cells in MAC biopsy specimens was in the range of 10% to 30% (Figure 5B).As shown in Figure 5C, the
quality of the model showing the dependence of MAC metastasis process in lymph nodes on
KIL-1β/IL1R2 was very good (AUC = 0.770). The AUC values for IL-1β (pg/mL),
IL1R2 (colored area, %), and KIL-1β/IL1R2 (conventional units) were,
respectively, 0.616, 0.226, and 0.770. It was found that at KIL-1β/IL1R2 ≤100
the percentage of patients with metastases was equal to 24.0%, at KIL-1β/IL1R2
≤25% to 36.7% and at KIL-1β/IL1R2 ≤5% to 50.0%. The quality of the ROC model
for the division of the patient group into a subgroup of patients without lymph node
metastases and, accordingly, into a subgroup of patients with metastases, based on the use
of indicators IL-1β and KIL-1β/IL1R2, markedly increased when taking into
account the indicators of only those patients (n = 31), in which the relative content of
highly differentiated tumor cells in MAC biopsy specimens was in the range of 10% to 30%.
The value of AUC has increased by almost 30% (AUC = 0.910), and its quality has acquired
the status of “excellent model” (Figure
5D).
Correlation Between CSF2RA and IL1R2 Expression, KGM-CSF/CSF2RA, and
KIL-1β/IL1R2 Coefficients and Cytokine Concentrations in the MAC Culture
Supernatants
To determine the specific features of cytokine regulation of CSF2RA and GM-CSF and IL1R2-
and IL-1β–dependent pathways of tumor cell activation, an analysis of correlation was
performed on not only CSF2RA and IL1R2 expression in the samples but also on the secretion
levels of a set of cytokines in the culture supernatants of the corresponding MAC samples
(Table 2). When we studied
the association between receptor CSF2RA expression and cytokine concentration in the tumor
culture supernatant, we found only 1 correlation between CSF2RA expression and the
expression of IL-1Ra (Table
2). Parameter KGM-CSF/CSF2RA showed a positive correlation with the
concentrations of IL-6, IL-8, IL-1Ra, and G-CSF in MAC culture supernatants. When we
studied the association between receptor IL1R2 expression in MAC and cytokine
concentrations in the tumor culture supernatant, we identified only 1 negative correlation
between IL1R2 expression and IFN-γ concentration (Table 2).
Table 2.
Coefficients (r) of Correlation of CSF2RA Expression, IL1R2
Expression, KGM-CSF/CSF2RA, and KIL-1β/IL1R2 With Cytokine
Concentrations in MAC Culture Supernatants.
Coefficients (r) of Correlation of CSF2RA Expression, IL1R2
Expression, KGM-CSF/CSF2RA, and KIL-1β/IL1R2 With Cytokine
Concentrations in MAC Culture Supernatants.Abbreviations: G-CSF, granulocyte colony-stimulating factor; GM-CSF, granulocyte
macrophage colony-stimulating factor; IFN-γ, interferon γ; IL, interleukin; MAC,
mammary adenocarcinoma; TNF-α, tumor necrosis factor α; VEGF-A, vascular endothelial
growth factor A.In contrast, when we studied the association between coefficient KIL-1β/IL1R2
and cytokine concentrations in the tumor culture supernatant, 2 positive correlations—with
IL-1β and IFN-γ concentrations—and 2 negative correlations were found: with VEGF-A and
TNF-α concentrations in MAC culture supernatants.
Discussion
It is known that any cytokines can act directly only on those target cells that express
their corresponding receptors.[15,16] This mechanism also works in the interaction of tumor cell receptors with
complementary cytokines. According to the published data, the L1R2 receptor for IL-1b and
CSF2RA for GM-CSF can be expressed on neutrophils, monocytes, polarized M2 macrophages, some
regulatory T cells, and B cells.[17-22] Moreover, according to the information in The Human Protein Atlas (an international
scientific database), some tumor cells of breast cancer can express IL1R2 (https://www.proteinatlas.org/ENSG
00000115590
-IL
1
R
2
/pathology/tissue/breast+cancer#img). At the same time, it was found that
IL-1b and GM-CSF are produced by different types of cells included in the microenvironment
of breast tumors (monocytes, macrophages, B-lymphocytes, endothelial cells) as well as
fibroblasts (GM-CSF) and directly by some breast cancer cells (IL-1b).[21-25]The data on the role of different cytokines in tumor progression and metastasis are
inconsistent and ambiguous, making it difficult to accurately predict the effects of
cytokine therapy in cancer, including breast cancer.[25-29] The ambiguousness of the effect of multiple cytokines on the tumor growth and
metastasis in different patients can be caused by various reasons: by different proportions
of tumor cells that express receptors interacting with the mediators that regulate tumor
growth and by different production levels of the corresponding cytokines. Based on this, it
follows that the search for biological predictive markers of metastasis is, first of all,
the search for key biological factors that are directly or indirectly related to many other
factors that affect the process of metastasis. In our work, data were obtained showing that,
as of such key factors may include variables such as KGM-CSF/CSF2RA and
KIL-1β/IL1R2, the value of that is correlated with several histopathological
parameters and level of production of many cytokines that can affect cytophysiological
characteristics of tumor cells (mitotic, migration, and hydrolytic activity), determining of
metastatic potential.In our study, the positive correlations found between KIL-1β/IL1R2 and the
concentrations of IL-1β in the culture supernatant suggest that an increase in the
production of IL-1β by the tumor is not associated with an increase in the expression of
IL1R2. A negative correlation is found between KIL-1β/IL1R2 and the
concentrations of VEGF-A. As known, VEGF-R2-mediated intracellular signals increase tumor
cell survival during hypoxia because of secretion of VEGF via an autocrine pathway, which
can contribute to the development of a more aggressive phenotype of tumor cells.[7] When VEGF-R2 is expressed by tumor cells, secreted VEGF can act as an autocrine
factor that triggers proliferation and increases their survival by blocking apoptosis.[7]It was shown that the increased production of GM-CSF in MAC (which is accompanied by a
decreased in CSF2RA expression) is associated with a reduction in the proportion (%) of
highly differentiated tumor cells. On the contrary, decreased production of IL-1β in MAC
(which is accompanied by an increase in IL1R2 expression) is associated with an increase in
the proportion of highly differentiated tumor cells and a decrease in the proportion of
poorly differentiated tumor cells. The observed positive correlation between the number of
mitoses in a tumor tissue sample and the KIL-1β/IL1R2 shows that proliferation of
tumor cells depends on the IL-1β–IL1R2 ratio in MAC. The data on the correlations between
CSF2RA and IL1R2 expression levels and KGM-CSF/CSF2RA and KIL-1β/IL1R2
on the one hand and cytokine concentrations in the culture supernatant of MAC samples on the
other hand can be interpreted as follows.A positive correlation between CSF2RA and IL-1Ra may indicate a stimulating effect of
antagonist IL-1Ra on CSF2RA expression in tumor cells (this effect is likely macrophage
mediated). A positive correlation of cytokines IL-6 and IL-8 with coefficient
KGM-CSF/CSF2RA also confirms the influence of the said cytokines on this
stimulating effect. The positive correlation between IL1R2 and IFN-γ found in our study
indicates a stimulating effect of IFN-γ on IL1R2 expression in tumor cells. The modifying or
regulatory effect of IFN-γ on the IL1R2- and IL-1β–dependent pathway of cell activation in
MAC is supported by the positive correlation between KIL-1β/IL1R2 and the IFN-γ
concentration in MAC culture supernatant. The correlation between KIL-1β/IL1R2
and the VEGF-A concentration probably means the importance of the IL1R2/IL-1β ratio for the
regulation of production of angiogenic factor VEGF-A, which is required for vascular growth
in the tumor, which in turn determines tumor growth and metastasis.From a practical and theoretical point of view, the results obtained by us with the help of
ROC analysis are important, which showed that KIL-1β/IL1R2 index is a fairly
significant complex biological marker that allows to identify a group of patients who have
no metastases to regional lymph nodes. With the help of ROC analysis, we also showed that
KIL-1β/IL1R2 is a biological marker, allowing additional consideration of the
number of differentiated forms of tumor cells in MAC with even greater probability to
identify a group of patients who have no metastases in the regional lymph nodes. This is
very important from a practical point of view. Oncologists often recommend the removal of
lymph nodes after the diagnosis of cancer. However, the feasibility of excision of all
regional lymph nodes in any form of malignant tumors in the mammary glands has recently been
questioned.In conclusion, this study showed the feasibility of detecting KIL-1β/IL1R2 index
as fairly significant complex biological marker that allows to identify a group of patients
who have no metastases to regional lymph nodes. We found a number of correlations of various
histopathological parameters (that characterize the grade of MAC) with
KIL-1β/IL1R2, KGM-CSF/CSF2RA, CSF2RA, and IL1R2 expression, and a
number of correlations of KIL-1β/IL1R2, KGM-CSF/CSF2RA, CSF2RA, and
IL1R2 expression. The revealed correlations can allow to understand some mechanisms of
immunological influence on the process of tumor growth and metastasis, to outline further
ways of studying these mechanisms.
Authors: A J Marrogi; A Munshi; A J Merogi; Y Ohadike; A El-Habashi; O L Marrogi; S M Freeman Journal: Int J Cancer Date: 1997-10-21 Impact factor: 7.396
Authors: Emad A Rakha; Jorge S Reis-Filho; Frederick Baehner; David J Dabbs; Thomas Decker; Vincenzo Eusebi; Stephen B Fox; Shu Ichihara; Jocelyne Jacquemier; Sunil R Lakhani; José Palacios; Andrea L Richardson; Stuart J Schnitt; Fernando C Schmitt; Puay-Hoon Tan; Gary M Tse; Sunil Badve; Ian O Ellis Journal: Breast Cancer Res Date: 2010-07-30 Impact factor: 6.466
Authors: Alexander Autenshlyus; Sergey Arkhipov; Elena Mikhailova; Igor Marinkin; Valentina Arkhipova; Ekaterina Mogilnaya; Nikolay Varaksin; Michael Rukavishnikov Journal: Int J Immunopathol Pharmacol Date: 2017-07-26 Impact factor: 3.219
Authors: Zhe Wang; Shiyi Yang; Yusuke Koga; Sean E Corbett; Conor V Shea; W Evan Johnson; Masanao Yajima; Joshua D Campbell Journal: NAR Genom Bioinform Date: 2022-09-13
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