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HomeMILLIPLEX® Multiplex for Luminex® ImmunoassaysCorrelation of Angiogenesis Biomarkers with Early Metastatic Progression in NSCLC Through a Multiplex Immunoassay

Correlation of Angiogenesis Biomarkers with Early Metastatic Progression in NSCLC Through a Multiplex Immunoassay

With the angiogenesis pathway being complex and containing numerous targets to analyze, simultaneous quantification of multiple biomarkers, such as through the use of the MILLIPLEX® Human Angiogenesis/Growth Factor Panel 1, saves valuable resources. Read on to learn how this panel was used to correlate angiogenesis biomarkers with early metastatic progression in NSCLC.

What is Angiogenesis?

Angiogenesis is a fundamental process in growth, development, and tissue repair. It involves the underlying vascular infrastructure crucial to the delivery of nutrients that is created by a well-studied combination of growth factors and regulatory elements. Dysregulation of this process leads to abnormal blood vessel growth involved in many common diseases and plays a significant role in tumor growth and metastasis.

How Does Angiogenesis Relate to Cancer?

In many types of cancer, aberrations in regulatory signaling pathways lead to sustained angiogenesis, a necessary component fueling the ability of cancerous tissue to thrive via continuous unregulated replication 1,2. The process of angiogenesis is normally a tightly regulated balance between pro-angiogenic growth factors (VEGF, FGF, PDGF, TGF) and anti-angiogenic signaling molecules (thrombospondin, angiostatin, and endostatin), along with complex membrane-bound receptors and endothelial cell interactions1,2. Malignant cells, however, sway this delicate equilibrium, resulting in rapid vascular growth with various underlying structural and functional abnormalities. From an investigative and therapeutic standpoint, it is important to identify and subsequently target the growth factors or regulatory elements that play crucial roles in allowing angiogenic dysregulation. With the overwhelming numbers of these targets for potential investigation, it is a challenge to decide among them and efficiently quantitate multiple targets.

Using Multiplex Immunoassays to Analyze Angiogenesis Biomarkers

Current detection assays are limited by minimal automation, low overall output, and excessive cost. To quickly and affordably identify specific angiogenic processes, it is necessary to screen large panels of vascular analytes and growth factors with some level of automation or high throughput.

The utility of the MILLIPLEX® Human Angiogenesis/ Growth Factor Magnetic Bead Panel 1 in the analysis of 17 targets involved in the angiogenesis pathway was determined in a cohort of 38 patients with various stages of non-small cell lung cancer (NSCLC). The objective was to determine if the MILLIPLEX® assay can accurately quantify known angiogenesis targets in a practical, high-throughput fashion.

Methods

Patient Cohort

Serum was collected from a total of 38 patients with pathologically confirmed NSCLC between 2004 and 2008 at Rush University Medical Center in Chicago, IL. Full Institutional Review Board approval was obtained for this study, and patient consents are on record for all participants. Twelve patients were pathologically staged3 as T1-2N0M0 (“no metastatic progression”), 12 with T1-3N1-2M0 (“locally-advanced”), and 14 patients with T1-4N1-2M1 disease (“presence of distant metastases”). All patients were not previously treated with either chemo- or radiotherapy.

Sample Preparation

Serum was processed from whole blood using conventional methods within an hour of venipuncture and archived at -80 °C. No sample was subjected to more than two freeze/thaw cycles for this study. Frozen samples were thawed completely at 4 °C, mixed by vortexing, and centrifuged at 10,000 x g for 10 minutes to remove particulates. All samples were diluted at 1:3 in the provided assay buffer solutions, as recommended in the MILLIPLEX® assay kit protocols.

Immunoassay Protocol

The Human Angiogenesis/Growth Factor Magnetic Bead Panel 1 was used to quantify the following 17 human angiogenesis and growth factor biomarkers: Angiopoietin-2, BMP-9, EGF, Endoglin, Endothelin-1, FGF-1 (acidic FGF), FGF-2 (basic FGF), Follistatin, G-CSF, HB-EGF, HGF, IL-8, Leptin, PLGF, VEGF-A, VEGF-C, and VEGF-D.

Antibody-conjugated magnetic beads were prepared by sonicating for 30 seconds, then vortexing for 1 minute. All samples, quality control samples, and standards were prepared as recommended in the MILLIPLEX® assay kit protocols with supplied diluents and processed in duplicate batches. The protocol was as follows:

  • 200 μL of assay buffer was added to each well and decanted.
  • 25 μL of each sample and 25 μL of prepared beads were then added into appropriate wells, along with buffering solutions.
  • The plate was subsequently sealed and incubated overnight at 4 °C.
  • The plates were washed 3 times and followed by the addition of 25 μL detection antibodies into each well.
  • After 1-hour incubation at room temperature, 25 μL of Streptavidin-Phycoerythrin was added to each well and incubated for an additional 30 minutes at room temperature.
  • The plates were washed 3 times and finally resuspended in 100 μL of sheath fluid in each well.
  • The assay plate was then analyzed with the Luminex® instrument equipped with xPONENT® software.

Statistical processing was accomplished in SPSS v15.0 and Microsoft Office Excel® 2007. Clinical outcomes were assessed by log-rank and Kaplan-Meier estimates of median time to recurrence using the R statistical software package.

Multiplexing Results

As described above, the angiogenesis multiplex panel was used to quantify 17 analytes relevant to angiogenesis in clinical specimens representative of the different stages of disease progression in NSCLC. As seen in both Table 1 and Figure 1, the results showed superb assay precision across a wide range of analyte concentrations.

Table 1. The %CVmean was calculated by averaging %CV values for each standard across the 8-point standard range (including 0 point). Levels for the angiogenesis biomarkers were determined based on the 7-point standard curve suggested by the MILLIPLEX® assay kit protocol and provided a wide dynamic range for each analyte (Figure 1). This dynamic range enabled most targets to be readily measured in human serum.
Graphs showing the standard curves for each analyte measured by the MILLIPLEX® Human Angiogenesis/Growth Factor Magnetic Bead Panel 1 (Cat. No. HAGP1MAG-12K). (Note: MFI = Median Fluorescence Intensity.)

Figure 1.Standard curves for each analyte measured by the MILLIPLEX® Human Angiogenesis/Growth Factor Magnetic Bead Panel 1. (Note: MFI = Median Fluorescence Intensity.)

Results showed comparable performance characteristics in the patient samples, as shown in Table 2.

Table 2. Analysis of 3 cohorts of NSCLC patients with the MILLIPLEX® Human Angiogenesis/Growth Factor Magnetic Bead Panel 1. (Note: All values are provided in pg/mL.)

Based on the cohorts tested, significantly higher expression of IL-8, HGF, and HBEGF in serum was observed from patients with “distant metastases”/ disseminated disease, as compared to serum from patients with no metastases (Table 2, Figure 2). These trends were consistent with previous work produced by this laboratory, that varying expression of growth factors and other signaling molecules likely involved in the angiogenesis pathway exist and may predict tumor metastasis4.

Graphs showing expression levels of analytes from NSCLC samples. IL-8, HB-EGF, and HGF are more highly expressed in NSCLC patients with metastatic disease.

Figure 2.IL-8, HB-EGF, and HGF are more highly expressed in NSCLC patients with metastatic disease. Box-and-whisker plots illustrate the range of each cohort for IL-8, HGF, and HB-EGF. T1-2N0M0 represents “no metastatic progression,” T1-3N1-2M0 represents “locally advanced” disease that is confined to the locoregional lymph nodes, and T1-4N1-2M1 represents the presence of “distant metastases” or disseminated disease. The following statistical trends were calculated: IL-8, p=0.001 was calculated for T1-2N0M0 versus T1-4N1-2M1; HGF, p=0.004 was calculated for T1-2N0M0 versus T1-4N1-2M1; and for HB-EGF, p=0.004 was calculated for T1-2N0M0 versus T1-4N1-2M1, and p=0.005 for T1-2N0M0 versus T1-3N1-2M0. Please note that all outliers and extreme values were removed for the box plots shown.

When these measured values were evaluated by a Mann-Whitney Rank Sum test in relation to the clinical groups evaluated, several biomarkers correlated with the progression of the disease to the locoregional lymph nodes (see Figure 2). Multiple markers (e.g., EGF, PLGF, VEGF-A, and VEGF-C) trended towards significance. However, significance was not reached due to the low number of patients involved in this study. Interestingly, the patterns observed only provided insights into the early stages of metastatic progression and provided few insights into biological processes necessary for the distant spread of the tumor.

Given the findings presented previously, the focus was put on the T1-2N0M0 and T1-3N1-2M0 groups in terms of clinical outcome measures. Specifically, the median time to recurrence in relation to biomarker concentrations was evaluated using the median value for each biomarker as the threshold (see Figure 3). A total of 9 biomarkers were found with a log-rank p-value less than 0.05. Not shown in Figure 3 are BMP-9, Follistatin, HB-EGF, Angiopoietin-2, and VEGF-C. These data may provide important insights into clinically relevant biological changes that are mechanistically implicated in disease recurrence.

Graphs showing the Kaplan-Meier estimates of the median time to recurrence. Clinical outcomes for the T1-2N0M0 (“no metastatic progression”) and T1-3N1-2M0 (“locally advanced”) groups were evaluated via log-rank analysis for each of the 17 biomarkers for the median time to recurrence.

Figure 3.Kaplan-Meier estimates of the median time to recurrence. Clinical outcomes for the T1-2N0M0 (“no metastatic progression”) and T1-3N1-2M0 (“locally advanced”) groups were evaluated via log-rank analysis for each of the 17 biomarkers for the median time to recurrence. Shown above are the Kaplan-Meier curves for (A) FGF-2 [p=0.049], (B) VEGF-D [p=0.009], (C) HGF [p<0.001], and (D) PLGF [p=0.010]. Purple lines represent patients with values less than measured median concentrations, whereas the cyan lines represent values larger than the measured median concentrations.

Summary

These findings are illustrative of the general practical ability of this MILLIPLEX® assay kit to generate information that can directly enhance studies of cancer metastasis. Because the angiogenesis pathway being studied here is so complex and with so many targets to analyze, simultaneous quantification of multiple analytes, such as that provided by the MILLIPLEX® Human Angiogenesis/Growth Factor Magnetic Bead Panel 1, conserves valuable resources. This panel accurately measured multiple angiogenesis biomarkers relevant to this research. By selecting combinations of analytes within the panel, any researcher can easily customize the panel to answer specific research questions.

This research was conducted at Rush University Medical Center in Chicago, IL. Data was provided by Jeffrey A. Borgia, Ph.D., Daniel Rinewalt, M.D., Cristina Fhied, M.S., and Michael J. Liptay, M.D. in 2018.

Materials
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For Research Use Only. Not For Use In Diagnostic Procedures.

References

1.
Winder T, Lenz H. 2010. Vascular Endothelial Growth Factor and Epidermal Growth Factor Signaling Pathways as Therapeutic Targets for Colorectal Cancer. Gastroenterology. 138(6):2163-2176. https://doi.org/10.1053/j.gastro.2010.02.005
2.
Carmeliet P, Jain RK. 2011. Molecular mechanisms and clinical applications of angiogenesis. Nature. 473(7347):298-307. https://doi.org/10.1038/nature10144
3.
Rami-Porta R, Crowley J, Goldstraw P. 2009. The revised TNM staging system for lung cancer. Ann Thorac Cardiovasc Surg. Feb;15(1):4-9. https://pubmed.ncbi.nlm.nih.gov/19262443/
4.
Farlow EC, Vercillo MS, Coon JS, Basu S, Kim AW, Faber LP, Warren WH, Bonomi P, Liptay MJ, Borgia JA. 2010. A multi-analyte serum test for the detection of non-small cell lung cancer. Br J Cancer. 103(8):1221-1228. https://doi.org/10.1038/sj.bjc.6605865
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