Diabetic Foot Clinical Trial
Official title:
Role of Adiponectine in Pathophysiology Ogf Diabetic Foot
Diabetic patients with a history of diabetic foot are considered to be a high-risk
population for increased cardiovascular and all-cause mortality (1,2,3,). Diabetic foot (DF)
is responsible for more hospitalizations than any other complication of diabetes and are the
leading cause of non-traumatic lower extremity amputations, resulting in nearly 100 000
amputations annually in the US alone (4,5,6). Surgical debridement, as an important
component of standard of care of diabetic foot, is intended to remove healing-impaired
tissue, decreases bacterial burden, thus to stimulate overall wound closure, while removing
as little of healing-competent skin as possible. Furthermore, debrided tissue is often used
as a valuable tissue source for research purposes (7,8,9,10). Debrided tissue presents
valuable diagnostic and research source to verify pathology, assess prognosis and gain
insights into DF molecular pathology, all of which ultimately leads to improved outcomes.
We aimed to validate tissue obtained from surgical debridement of DF for the
cellular/molecular tissue analyses and biomarkers, to evaluate the pathophysiology of DF and
understanding mechanisms that inhibit healing.
The age range will be 50-70 years, in order to minimize the effects of irreversible vascular
wall changes induced progressively by the aging process. All patients will undergo screening
procedures that will include full anamnesis, physical examination, basic laboratory blood
tests (full chemistry, CBC); urine examination and EKG will be performed at start and at the
end of the study. Patients with a significant myocardial, and renal, cerebrovascular or
hepatic disease will be excluded from the study.
In a prospective study, we will collect wound edge tissue specimens from 75 patients with DF
during surgical debridement. From each patient, 1-4 specimens will be obtained per
debridement. To evaluate debrided tissue, each specimen will be processed for paraffin
embedding and stained with haematoxylin and eosin. Histopathology analysis of multiple
specimens acquired from the same wound will be analysed.
Diabetic patients with a history of diabetic foot are considered to be a high-risk
population for increased cardiovascular and all-cause mortality (1,2,3,). Diabetic foot (DF)
is responsible for more hospitalizations than any other complication of diabetes and are the
leading cause of non-traumatic lower extremity amputations, resulting in nearly 100 000
amputations annually in the US alone (4,5,6). Surgical debridement, as an important
component of standard of care of diabetic foot, is intended to remove healing-impaired
tissue, decreases bacterial burden, thus to stimulate overall wound closure, while removing
as little of healing-competent skin as possible. Furthermore, debrided tissue is often used
as a valuable tissue source for research purposes (7,8,9,10). Debrided tissue presents
valuable diagnostic and research source to verify pathology, assess prognosis and gain
insights into DF molecular pathology, all of which ultimately leads to improved outcomes.
We aimed to validate tissue obtained from surgical debridement of DF for the
cellular/molecular tissue analyses and biomarkers, to evaluate the pathophysiology of DF and
understanding mechanisms that inhibit healing.
The age range will be 50-70 years, in order to minimize the effects of irreversible vascular
wall changes induced progressively by the aging process. All patients will undergo screening
procedures that will include full anamnesis, physical examination, basic laboratory blood
tests (full chemistry, CBC); urine examination and EKG will be performed at start and at the
end of the study. Patients with a significant myocardial, and renal, cerebrovascular or
hepatic disease will be excluded from the study.
In a prospective study, we will collect wound edge tissue specimens from 75 patients with DF
during surgical debridement. From each patient, 1-4 specimens will be obtained per
debridement. To evaluate debrided tissue, each specimen will be processed for paraffin
embedding and stained with haematoxylin and eosin. Histopathology analysis of multiple
specimens acquired from the same wound will be analysed. Full-thickness epidermis biopsies
will be followed by biomarker assessment such as:
1. Expression of insulin-like growth factor 1 receptor (IGF-1R)
2. Adiponectin
3. Leptin
4. Resistin
5. Osteocalcin
6. Osteoprotegerin
7. Insulin, c-peptid
8. HOMA-IR Blood sampling for chemistry and metabolic markers including lipids, fasting
glucose, fasting insulin, HbA1C, HOMA-IR , CRP, plasma adiponectin, visfatin, resistin,
and plasma leptin will be performed. Additionally, relationship between serum and
tissue adipokines level will be evaluated.
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