Andronikashvili Institute of Physics Department of Physics of Biological Systems [email protected]

Ni(II)

Ac-Glu-Ser-His-His-Amid (C-terminus fragment of H2A) Cu(II) and Ni(II)

Zinc is a novel intracellular second messenger like Ca 2+ and cAMP

B
(positively charged)

The double life of HMGB1 chromatin protein: Architectural factor and extracellular signal

HMGB1 is ubiquitous and only 10 times less abundant than core histones.

The cytokine-inducing activity resides in the B Box domain

The A Box antagonizes HMGB1- induced inflammation

HMGB1 can be exracellularly released by passive secretion from any necrotic cell or by active secretion from activated macrophages/monocytes.

HMGB1 and diseases: Sepsis; Lung inflammation; Arthritis; Ischemic stroke; Tuberculosis -Mycobacterial infection induces the secretion of high-mobility group box 1 protein

Bactericidal activity of HMGB1 - functionally belongs to the growing family of antibiotic peptides (Box A???)

Fetal human lung fibroblasts were grown up to 80% confluency prior to chromium treatment at the concentration range from 2-30 (μM).

 2 h Cr(VI)+46 h

⚪ 24 h Cr(VI)

◻ 48 h Cr(VI)

 24 h Cr(VI) +24 h

Concentration of Cr(VI) (μM)

Dr Marina Abuladze

h

24 h

A

B

ROS level in control untreated and Cr(VI)-treated HLF cells

h

2 h 4 h 24 h 48 h

A

B

Dr Nino Asatiani

Cr(VI)

Mn-SOD

Cu,Zn-SOD

C 2h

C 2h

C 24 h

C 24 h

C 24 h

Peak Density (% of Control)

Mn-SOD

Mn-SOD

Cu,Zn-SOD

Cu,Zn-SOD

2 h

24 h

2 h

24 h

Mn-SOD

Mn-SOD

Cu,Zn-SOD

Cu,Zn-SOD

2 h

24 h

Mn-SOD

Mn-SOD

Cu,Zn-SOD

Cu,Zn-SOD

A

B

Kartvelishvili

reaction. The model Fenton reaction mixture contained 100 mM DMPO, 1 mM FeSO4, 100 mM H2O2, 50 mM sodium/potassium buffer pH 7.4 in a final volume 62.5 μl.

The time course of the ESR signal intensity in the model Fenton reaction in the presence of crude cell extracts of Cr(VI)-treated and untreated control L-41 cells. (A) - 2 μM Cr(VI) treatment; (B) - 20 μM Cr(VI) treatment. ◆- Control;  - 24 h of the cell growth under Cr(VI) action;  - 48 h of the cell growth under Cr(VI) action. Cr(VI) as potassium chromate was added to the cell culture at the 48 h of growth (80% of confluence). Protein concentration in ESR sample was 0.168 mg/ml.

acute ischemic stroke

Recently much research interest is focused on predictors of functional outcome in stroke. The development of early prognostic biochemical parameters is of great importance. Accumulating data suggest that MMPs have a deleterious role in stroke. The hypothesis to be tested in this project is that the profile of plasma matrix metalloproteinases MMP-2, MMP-9 and MMP-12 is changed (elevated) during the hyperacute stage of the disease, and it provides prognostic information for stroke severity, especially malignant middle cerebral artery infarct along with other inflammatory markers (plasma status of antioxidant defense system).
1.To assess quantitatively the level of MMP-2, MMP-9 and MMP-12 in the blood plasma of stroke patients in the first 24 hours after stroke.
2. To estimate the oxidant/antioxidant balance in the blood plasma of patients and healthy volunteers and develop it as the marker of the disease.
3. To measure the blood level of extracellular cytokine HMGB1 as the possible factor upregulating MMPs in human stroke.
4. To estimate the predictive role of the above-mentioned serological markers in development of malignant cerebral infarcts.
5. To estimate the predictive role of the above-mentioned serological markers in functional outcome after IS.

3D Structure of MMP structures - ProMMP-2-TIMP-2 complex.
Orange - propeptide
Green - catalitic domail
Pink -fibronectin domain
Blue - TIMP-2
One catalitic Zn;
one structural Zn;
Three calcium ions

Zn

Zn

тракт, уро-репродуктивный тракт)

Микрочип - это пластинка, покрытая тонким слоем фиксирующего нейтрального вещества (например модифицированного акриламида), в которое в совершенно определенной последовательности нанесены фрагменты ДНК (олигонуклеотиды), специфически сконструированные и синтезированные для диагностики.

Нуклеиновые кислоты (из ассоциированных со слизистой облочкой СРБ из биопсийного материала в случае больных ЯК и из крови в случае анализа TORCH-инфекции) выделяются и метятся флуоресцентными метками

диагностики бактериального происхождения язвенных колитов (ЯК) и для наблюдения за проходящим курсом лечения антибиотиками;
Больные и здоровые люди являются носителями сульфат редуцирующих бактерий (СРБ), однако профиль бактериальных популяций обнаруживает поразительное различие.
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