Identification of stromal ColXα1 and tumor-infiltrating lymphocytes as putative predictive markers of neoadjuvant therapy in estrogen receptor-positive/HER2-positive breast cancer

From the ER+/HER2+ patients we selected a mixture of good and poor responders for whom we had sufficient tissue for this assay. Ten micron tumor sections were scraped from the slides for total RNA extraction. RNA was purified using the RecoverAll Total Nucleic Acid Extraction Kits for FFPE tissues (Ambion, Austin, TX) and further purified and concentrated with the RNEasy Minelute Cleanup Kit (Qiagen, Valencia, CA).

RNA was isolated and purified using the RNeasy FFPE kit (Qiagen, Valencia, CA, USA). One hundred nanograms of total RNA was amplified using Affymetrix’ Sensation Plus FFPE amplification kit following the manufacturer’s instructions and labeled cDNA was hybridized to Affymetrix (Santa Clara, CA, USA) HTA 2.0 microarrays and visualized at the Brown University Genomics Core Facility following the manufacturer’s instructions. Signals were estimated using RMA [15]. Fold change, t-tests, and multiple hypothesis tests were calculated in R. Data are available in GEO, GSE67982.

For real-time qPCR, cDNA was prepared using QuantiTect Reverse Transcription Kit (Qiagen). qPCR was performed on a Mx3005p (Agilent) with Brilliant III SYBR Green (Agilent). Relative expression fold changes were calculated relative to GAPDH.

Microarray signals were analyzed for statistical significance in terms of differences between samples between good and poor responders. We applied gene set enrichment analysis (GSEA) to investigate pathways and groups of genes that may be associated with NAC response, which identified collagens and immune pathways as strongly associated with good pathologic response. The collagen transcript, Col10A1, was one of the top-ranked transcripts associated with NAC response for which an available commercial antibody was available. Collagen, type 10, alpha 1 (gene name Col10A1 and protein product ColXα1) is a secreted, homotrimeric short-chain collagen and is up-regulated in a variety of tumor types with restricted or undetectable expression in a large spectrum of normal tissues, normal primary cultures and tumor cell lines [7, 8]. After verification of the microarray observations by qPCR, we tested the association of ColXα1 expression as well as other tumor microenvironmental factors such as the abundance of tumor associated stroma and TILs in the pre-treatment biopsy samples to correlate with post-treatment response. TCGA RNA-seq data for breast invasive carcinoma were downloaded from the Firehose Broad GDAC [16]. TCGA clinical data were downloaded from the TCGA data archive in September 2015 (http://​cancergenome.​nih.​gov/​).

We morphologically evaluated the amount intratumoral stroma and TILs on pre-treated biopsy samples which commonly consisted of 2–5 needle cores of average 1.5 cm in length obtained with either a 14 gauge spring-loaded biopsy device or a 12 gauge vacuum-assisted biopsy device. The amount of intratumoral stroma was scored as 0 to 2: 0 for absent or minimal stroma (<10 %), 1 for mild to moderate amount of stroma (10–40 %) and 2 for abundant stroma (≥40 %). Stromal and intratumoral TILs (sTILs and iTILs) were evaluated based on criteria published by Denkert et al. [2]. Briefly, iTILs were defined as lymphocytes in direct contact with the tumor cells, whereas sTILs were defined as lymphocytes in the surrounding stroma, with the percent of the tumor or stromal volume comprised of infiltrating lymphocytes, as opposed to tumor or other stromal tissues, on an H&E stained biopsy section estimated by the reading pathologists, with results reported in increments of 10 (0–1 % was scored as 0, with all other estimates rounded up to the next highest decile - i.e., 11–20 % was scored as 20). sTILs and iTILs were totaled to calculate TILs. The trends were similar for each lymphocyte fraction (data not shown). sTILs were chosen to be analyzed as they were considered to the most consistent metric as recommended by the International TILs Working Group [17]. The histological evaluation was graded independently by two pathologists (YW and JX), who were blinded to clinical information including the post-treatment outcome, at the time of analysis, with the summary score representing the mean of the two separate scores. The two pathologists evaluated 30 separate cases (triple negative breast cancer cases) together to get a general agreement of the sTIL. The actual study cases were evaluated independently, the concordance is about 95 %. The cases with greater than 10 % difference were reviewed together and the average score was used.

Four-micron sections were cut from formalin-fixed paraffin-embedded tissue blocks, heated at 60 °C for 30 min, deparaffinized, rehydrated and subjected to antigen retrieval by heating the slides in epitope retrieval buffer in a water bath at 95 °C for 45 min. The slides were then incubated with either mouse monoclonal antibodies or rabbit polyclonal antibodies for 30 min at room temperature in a DAKO Autostainer. Anti- colXα1 (1:50, eBioscience/Affymetrix, Clone X53), estrogen receptor (1:50, DAKO (Santa Clara, CA, USA), clone 1D5), progesterone receptor (1:400, DAKO, clone 1A6), and HER2/neu (DAKO HercepTest^TM) were used for immunohistochemistry. The immunoreactivity was detected using the DAKO EnVision method according to the manufacturers recommended protocol. Peri- and intra-tumoral stromal staining for ColXα1 was scored as 0, 1+, 2+, and 3+. Briefly, 0 as no staining; 1+ as weak staining; 2+ as <10 % of stroma tissue with intense staining present; 3+ as >10 % of stroma tissue with patchy intense staining. All scoring was performed blinded to the outcome and many cases were scored before the outcome data was available.

SPSS v22 for MacOS (SPSS, Chicago, IL, USA) was used for all statistical analysis. P < 0.05 was considered statistically significant. All p-values reported are two-sided. For the logistic regression, all factors were analyzed as continuous variables.