Decreased HLA-DR antigen-associated invariant chain (CD74) mRNA expression predicts mortality after septic shock

The study group consisted of 93 septic shock patients (diagnostic criteria of the American College of Chest Physician/Society of Critical Care Medicine [7]) admitted to the surgical or medical ICUs of Lyon-Sud University hospital and who were alive three days after the onset of shock. The exclusion criteria were patients under the age of 18 years old, subjects with aplasia or immunosuppressive disease (for example, HIV) and patients that died before Day 3. Septic shock was defined by an identifiable site of infection, persisting hypotension despite fluid resuscitation requiring vasopressor therapy, and evidence of a systemic inflammatory response manifested by at least two of the following criteria: a) temperature >38°C or <36°C; b) heart rate >90 beats/minute; c) respiratory rate >20 breaths/minute; d) white blood cell count >12,000/mm³ or <4,000/mm³. Severity was assessed by the Simplified Acute Physiologic Score II (SAPS II) calculated at inclusion in the protocol. Development of organ dysfunction was assessed by the Sequential Organ Failure Assessment score (SOFA, range: 0 to 24) measured after 24 h of ICU stay. Mortality was defined as death occurring within 28 days after the onset of shock. The onset of septic shock was defined as the beginning of vasopressor therapy. In accordance with guidelines from the Surviving Sepsis Campaign and from our ICUs, septic shock patients were rapidly treated with empiric broad-spectrum antibiotherapy after admission.

Biological analyses were performed on residual blood after completing routine follow-up performed in the ICU. PAXgene® and EDTA-anti-coagulated tubes were collected at the same time from patients at Day 3 or Day 4 after diagnosis of septic shock. This work belongs to a global study on ICU-induced immune dysfunctions. It has been approved by our Institutional Review Board for ethics (“Comité de Protection des Personnes”) which waived the need for informed consent because this study was observational and biomarker expressions were measured on a very low volume of residual blood after completion of routine follow-up. This study is also registered at the French Ministry of Research and Teaching (#DC-2008-509) and recorded at the Commission Nationale de l’Informatique et des Libertés.

Circulating monocyte HLA-DR expression (mHLA-DR) was assessed by flow cytometry (NAVIOS; Beckman-Coulter, Miami, FL) as previously described [8]. Results are expressed as the number of antibodies bound per cells (AB/C).

Whole-blood mRNA expressions of five MHC-class II related genes (HLA-DRA, HLA-DMA, HLA-DMB, CIITA, CD74) were studied using blood samples collected directly in PAXgene blood RNA tubes (PreAnalytix, Hilden, Germany). Total RNA was extracted using the PAXgene Blood RNA kit (PreAnalytix). Before RNA elution, the residual genomic DNA was digested using the Rnase-Free Dnase set (Qiagen, Hilden, Germany). Total RNA was reverse transcribed into complementary DNA (cDNA) using SuperScript® VILO TM cDNA Synthetis (Life Technologies, Grand Island, NY). The gene panel constituting the MHC II was quantified using q- real time polymerase chain reaction. Polymerase chain reaction was performed in a LightCycler instrument using the standard Taqman Fast Advanced Master Mix PCR kit according to the manufacturer’s instructions (Roche Molecular Biochemicals, Basel, Switzerland). Thermocycling was performed in a final volume of 20 μL containing 5 μM of the required primers, 1 μM of required probe. PCR was performed with an initial denaturation step of 10 minutes at 95°C, followed by 45 cycles of a touchdown PCR protocol (10 sec at 95°C, 29 sec annealing at 68°C, and 1 sec extension at 72°C). The cDNA standards were prepared from purified PCR amplicons obtained with the corresponding primers (Table 1). The Second Derivative Maximum Method was used with the LightCycler software to automatically determine the crossing point for individual samples as previously described [1]. Standard curves were generated by using the quadruplicate cDNA standard. Relative standard curves describing the PCR efficiency of selected genes were created and used to perform efficiency-corrected quantification with the LightCycler Relative Quantification Software (Roche Molecular Biochemicals). Gene expression normalization was performed based on the combination of two selected housekeeping genes (HPRT1: hypoxanthine phosphoribosyltransferase 1 and GLYR1: glyoxylate reductase 1 homolog) and results were expressed as Calibrated Normalized Relative Quantity (CNRQ) [2]. Both reference genes (HPRT1 and GLYR1) were selected based on an ongoing project on reference genes usable in genomic studies in ICU patients. These were selected among a list of other reference genes based on their stability and the absence of differential expression between compared groups of patients. This analysis was performed by using the tools available via [9] (data not shown).

Comparisons between groups were made using the non-parametric Mann Whitney U-test (survivors vs non-survivors) for continuous variables and the Pearson chi-squared test, as appropriate, for categorical data. Correlation studies were performed with the Spearman’s rank correlation test. Receiver Operating Curves were performed to determine the cut-off values for CD74 mRNA or mHLA-DR expressions in regard to prediction of mortality. The best cut-off value was selected based on optimized Youden index. Using these thresholds, Kaplan-Meier survival curves were obtained and differences in survival between groups were evaluated using Log rank test. Uni- and multi-variate logistic regression analyses were used to identify the variables associated with death and Cox model permitted to estimate the Hazard Ratio and 95% confidence interval (CI 95%). Backward selection was used and a P-value of 0.05 was considered as statistically significant. Because SAPS II and SOFA scores confirmed the assumed linearity with the outcome (survivors vs non survivors), these variables were included in the model as continuous variables. Statistical analyses were performed with SPSS (version 17.0, SPSS, Chicago, IL, USA) and GraphPad Prism® (version 4.03, GraphPad Software, La Jolla, CA, USA) softwares.