Inflammation Clinical Trial
— EXPOCOLOfficial title:
The Influence of Breathing Techniques and Exposure to Cold on Inflammation During Human Endotoxemia, an Explorative Study'
NCT number | NCT03240497 |
Other study ID # | EXPOCOL |
Secondary ID | |
Status | Completed |
Phase | N/A |
First received | |
Last updated | |
Start date | April 12, 2016 |
Est. completion date | April 2018 |
Verified date | July 2017 |
Source | Radboud University |
Contact | n/a |
Is FDA regulated | No |
Health authority | |
Study type | Interventional |
Inflammatory cytokines play a pivotal role in rheumatoid arthritis (RA) and innovative
non-pharmacological therapies aimed at limiting cytokine production are highly warranted.
Recently, our group showed that healthy volunteers trained in an intervention developed by
'Iceman' Wim Hof were able to voluntarily attenuate the pro-inflammatory response during
experimental human endotoxemia (a model of systemic inflammation elicited by administration
of lipopolysaccharide [LPS] in healthy volunteers). Subjects trained in the intervention
exhibited profound increases in plasma adrenaline levels, a rapid increase of an
anti-inflammatory cytokine and subsequent attenuation of the pro-inflammatory response.
The intervention consists of three elements, namely meditation, exposure to cold and
breathing techniques. The meditation element is not likely to be involved. It was a very
minor part of the training program and was not practiced during the endotoxemia experiments.
Exposure to cold and the subsequent rewarming to normal body temperature may influence the
inflammatory response through the release of immunomodulatory molecules like HSP-70. Also,
exposure to cold can induce an ischemia-reperfusion-like state in the skin and peripheral
tissue that is known to be involved in the downregulation of pro-inflammatory cytokines and
upregulation of anti-inflammatory cytokines. The investigators anticipate that the third
element, breathing techniques, is the major contributor to the anti-inflammatory effects of
the intervention previously observed. The present study aims to explore the effects of the
breathing technique ('strength ventilation'), the exposure to cold, and these two elements
combined on the immune response during human endotoxemia. Elucidation of the relative
contribution of the elements is of importance to establish a feasible, safe, and effective
intervention for future use in patients.
Objective: The primary objective of the present study is to determine the effects of the
`strength ventilation` breathing technique and exposure to cold, both separately and in
combination, on the inflammatory response during human endotoxemia. To this end, a 2 by 2
design will be employed. Additionally, an evaluation of the influence of the cold exposure
and breathing technique on pain thresholds and oxygen tension in the mitochondria will take
place.
Status | Completed |
Enrollment | 48 |
Est. completion date | April 2018 |
Est. primary completion date | April 2018 |
Accepts healthy volunteers | Accepts Healthy Volunteers |
Gender | Male |
Age group | 18 Years to 35 Years |
Eligibility |
Inclusion Criteria: - Written informed consent - Male - Healthy Exclusion Criteria: - Prior experience with any of the elements of the intervention developed by Hof - Prior experience with other breathing, meditation, or cold exposure techniques - Prior experience with mindfulness or yoga - Prior experience with exposure to cold showers - Frequent visits to sauna facilities (more than 1/month) - Use of any medication - Smoking - History of asthma - History of porphyria - Previous spontaneous vagal collapse - History of atrial or ventricular arrhythmia - (Family) history of myocardial infarction or stroke under the age of 65 years - Cardiac conduction abnormalities on the ECG consisting of a 2nd degree atrioventricular block or a complex bundle branch block - Hypertension (defined as RR systolic > 160 or RR diastolic > 90) - Hypotension (defined as RR systolic < 100 or RR diastolic < 50) - Renal impairment (defined as plasma creatinin >120 µmol/l) - Liver enzyme abnormalities - Medical history of any disease associated with immune deficiency - CRP > 20 mg/L, WBC > 12x109/L, or clinically significant acute illness, including infections, within - 4 weeks before endotoxin administration - Participation in a drug trial or donation of blood 3 months prior to the LPS challenge - Use of recreational drugs within 7 days prior to endotoxemia experiment day - Recent hospital admission or surgery with general anaesthesia (<3 months) |
Country | Name | City | State |
---|---|---|---|
Netherlands | Radboud University Medical Centre, Intensive Care | Nijmegen |
Lead Sponsor | Collaborator |
---|---|
Radboud University | Erasmus Medical Center |
Netherlands,
Type | Measure | Description | Time frame | Safety issue |
---|---|---|---|---|
Primary | circulating TNF-a | The main study endpoint is the difference in circulating TNF-a over time following LPS administration between groups | 8 hours | |
Secondary | Cytokines | Levels of other circulating cytokines (including, but not limited to IL-6, IL-10 and IL-1RA) | 8 hours | |
Secondary | Plasma adrenaline levels | routine analysis methods also used for patient samples (high-performance liquid chromatography with fluorometric detection | 8 hours | |
Secondary | Plasma cortisol levels | routine analysis methods also used for patient samples performed by the Department of Laboratory Medicine of the Radboud University Nijmegen Medical Centre. | 8 hours | |
Secondary | - Blood gas parameters | Blood gas parameters will be analyzed using the i-STAT Blood Gas Analyzer (Abbot, Hoofddorp, The Netherlands). | 8 hours | |
Secondary | - Mitochondrial oxygen tension | The COMET device measures cutaneous mitochondrial oxygen tension (MitoPO2) over time. MitoPO2 is measured by means of delayed fluorescence of mitochondrial protoporphyrin IX (PpIX) [6]. Microcirculatory flow can be stopped by applying pressure with the measuring probe on the skin, enabling the determination of the oxygen disappearance rate (ODR) | 8 hours | |
Secondary | - Metabolome | The metabolome will determined using the `Kenkodo @home` sampling set, developed by Metabolomic Discoveries GmbH (http://www.metabolomicdiscoveries.com/). Using a minimally invasive finger prick we will obtain 10µl (microliter) of blood from the subjects. The used Mitra Sampling Device is a Class 1 medical device (D254956) and complies with FDA good manufacturing practices. Samples will be analyzed at Metabolomic Discoveries GmbH. |
8 hours | |
Secondary | - Body temperature | The course of body temperature will be determined every 30 minutes for the first 8 hours after endotoxine administration using an infrared tympanic thermometer (Sherwood Medical, `s-Hertogenbosch, the Netherlands). | 8 hours | |
Secondary | - Illness score | To monitor the onset and alterations of endotoxine-induced symptoms, all subjects will be asked to score the severity of nausea, headache, shivering, muscle- and backpain every 30 minutes during the course of the experiment. Symptoms are scored on a scale ranging from 0 (symptom not present) to 5 (symptom is worst ever experienced). | 8 hours | |
Secondary | heart rate | Heart rate will be continuously measured by connecting the arterial catheter to an arterial pressure monitoring set. Data will be recorded from the patient monitor every 30 seconds by a custom in-house-developed data recording system. | 8 hours | |
Secondary | Blood pressure | Blood pressure will be continuously measured by connecting the arterial catheter to an arterial pressure monitoring set. Data will be recorded from the patient monitor every 30 seconds by a custom in-house-developed data recording system. | 8 hours | |
Secondary | - Leukocyte counts and differentiation | Measurements of haemoglobin, leukocyte and thrombocyte count, determinations of kidney and liver function, amylase, CRP, cortisol and catecholamines will be performed by the laboratory for clinical chemistry at the Radboud university medical center. | 8 hours | |
Secondary | Pain thresholds: PPT | PPT will be measured on the left and right bodyside once at three locations. Single pulse evoked pain measurement is performed by one pulse at 150% of the EPT and assessed on a VAS. . | 8 hours | |
Secondary | Pain thresholds: EPTT | Electrical Pain Tolerance Thresholds (EPTT) (test stimulation) are assessed and expressed in milli-Ampère on the m. Rectus femoris contralateral to the dominant hand | 8 hours | |
Secondary | - Presence of TLR ligands in plasma | HSP70 will be measured in using ELISA. Presence of other TLR ligands in plasma will be studied using transfected HEK-blue TLR cells (Invivogen). | 8 hours | |
Secondary | - HSP70 levels in plasma. | HSP70 will be measured in using ELISA. Presence of other TLR ligands in plasma will be studied using transfected HEK-blue TLR cells (Invivogen). | 8 hours | |
Secondary | - Production of inflammatory mediators by ex vivo-stimulated leukocytes | Ex vivo leukocyte stimulation by different pathogens will be performed at the Laboratory of General Internal Medicine of the Radboud university medical center. Cytokines in supernatants of stimulated leukocyte cultures will be determined by ELISA. Inflammatory transcriptional pathways will be determined by quantitative PCR/microarrays/RNA sequencing at the Laboratory of General Internal Medicine of the Radboud university medical center and/or the University of Groningen medical center. | 8 hours | |
Secondary | - Inflammatory transcriptional pathways sequencing | by use of qPCR/microarrays/RNA | 8 hours |
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