Post on 26-Mar-2015
Alcohol Dehydrogenase I is Alcohol Dehydrogenase I is Present in Normal Human Present in Normal Human
Mammary Tissue and Absent Mammary Tissue and Absent in Breast Cancer: in Breast Cancer:
Implications for Breast Implications for Breast CarcinogenesisCarcinogenesis
Trudy A. Atkins, M.S.Trudy A. Atkins, M.S.Supervisor of Science and G & T EducationSupervisor of Science and G & T Education
East Brunswick Public SchoolsEast Brunswick Public Schools
December 20, 2011December 20, 2011
Retinol
Alcohol Dehydrogenase
Retinal
A
ldheh
yde
Dehyd
rogen
ase
Retinoic Acid
NAD+ NADH
NADPHNADP+
NAD+
NADH
Alcohol Dehydrogenase
ββ-Carotene Retinol Retinoic -Carotene Retinol Retinoic AcidAcid
Functions of RetinolFunctions of Retinol
Vision Vision Bone GrowthBone Growth Cell DivisionCell Division Cell DifferentiationCell Differentiation Epi / Endothelial Maintenance Epi / Endothelial Maintenance
Nuclear Regulation by Retinoic Nuclear Regulation by Retinoic AcidAcid
Retinoic Acid Retinoic Acid Receptor – RARReceptor – RAR
Retinoid X Retinoid X Receptors – RXRReceptors – RXR
RAR/RAR RAR/RAR HomodimerHomodimer
(Chambon – 1987)(Chambon – 1987) RXR/RXR RXR/RXR
HomodimerHomodimer
(Manglesdorf – (Manglesdorf – 1990)1990)
RAR/RXR RAR/RXR HeterodimerHeterodimer
Retinoid SignalingRetinoid Signaling
Alcohol Dehydrogenase Alcohol Dehydrogenase IsozymesIsozymes
Five Classes – Five Classes – II, II, III, , II, III, IVIV, V, V DimericDimeric CytoplasmicCytoplasmic Zinc-dependantZinc-dependant Chromosome 4q22-24Chromosome 4q22-24
ADH IADH I
Dimeric – Composed of identical or non-identical Dimeric – Composed of identical or non-identical polypeptide chains alpha, beta, gamma.polypeptide chains alpha, beta, gamma.
Each polypeptide chain is 374 amino acids longEach polypeptide chain is 374 amino acids long 40 kD40 kD Two domains: catalytic and coenzyme bindingTwo domains: catalytic and coenzyme binding Functions in ethanol oxidation in liver, retinol Functions in ethanol oxidation in liver, retinol
oxidation in epithelium, oxidation of oxidation in epithelium, oxidation of
33ββ-hydroxysteroids-hydroxysteroids
Space Filling Model of ADH ISpace Filling Model of ADH I
ADH I ADH I (Alpha-blue / Beta 1-yellow)(Alpha-blue / Beta 1-yellow)
ADH IV – PurpleADH IV – PurpleADH I Beta - MustardADH I Beta - Mustard
ADH FamiliesADH Families
Associated Tumor Suppressor Associated Tumor Suppressor GenesGenes
p53p53 – Induces apoptosis by inducing IGFR I – Induces apoptosis by inducing IGFR I and its binding protein IGF-BP3. RA and its binding protein IGF-BP3. RA increases IGF-BP3 thereby increasing increases IGF-BP3 thereby increasing apoptosis in MDA-MB231 breast cancer apoptosis in MDA-MB231 breast cancer cell lines.cell lines.
c-mycc-myc – Over expressed in cancer cells. – Over expressed in cancer cells. RA acts to down-regulate this gene in MCF-RA acts to down-regulate this gene in MCF-7 breast cancer cell lines.7 breast cancer cell lines.
Breast AnatomyBreast Anatomy
Lobules – Lobules – Epithelium with Epithelium with surrounding surrounding myoepitheliummyoepithelium
Ducts - EpitheliumDucts - Epithelium Stroma – Stroma –
Connective Connective
Specific Aims:Specific Aims:
Western Blotting was used to determine if Western Blotting was used to determine if ADH I was located in normal breast ADH I was located in normal breast epithelium.epithelium.
Enzyme assays were performed in order to Enzyme assays were performed in order to determine the presence of ADH I in normal determine the presence of ADH I in normal breast epithelium and in breast cancerbreast epithelium and in breast cancer
Immunocytochemistry was used to determine Immunocytochemistry was used to determine the localization of ADH I in epithelial, the localization of ADH I in epithelial, myoepithelial, and stromal cells in normal and myoepithelial, and stromal cells in normal and malignant tissue.malignant tissue.
ResultsResults
Western BlotWestern Blot
Enzyme AssayEnzyme Assay
ImmunocytochemistryImmunocytochemistry
Initial ADH I Western BlotInitial ADH I Western Blot
CA = Cancerous tissue
N = Normal
F = Fibrocystic Tissue
ADH I with GAP (GTPase ADH I with GAP (GTPase Activating Protein) as a 5 µg Activating Protein) as a 5 µg
loading control loading control
Details of Western BlotDetails of Western Blot
ADH I – 40 kDaADH I – 40 kDa Asterisks indicate Asterisks indicate
protein from protein from “cancer” samples“cancer” samples
Note far right Note far right asterisk-lack of 40 asterisk-lack of 40 kDa band with kDa band with abundance of GAP abundance of GAP
Enzyme AssayEnzyme Assay Normal versus cancer oxidation of ethyl Normal versus cancer oxidation of ethyl
alcohol alcohol by ADH I.by ADH I. Duplicate samples with or without Duplicate samples with or without 4-methylpyrazole (4-MP) a known inhibitor of 4-methylpyrazole (4-MP) a known inhibitor of ADH I.ADH I. Change in absorbance was monitored on a Change in absorbance was monitored on a
dual beam spectrophotometer against a dual beam spectrophotometer against a reaction containing no substrate.reaction containing no substrate.
Enzyme activity is expressed as mIU/min/mg Enzyme activity is expressed as mIU/min/mg protein.protein.
N.D. indicates no detectable activity.N.D. indicates no detectable activity.
Enzyme Assay Enzyme Assay Normal vs. CancerNormal vs. Cancer
Normal Breast Breast Cancer
4-MP 4-MP Patient # Without With
Δ % Inhibition
Patient # Without With
Δ % Inhibition
N1 3.89 0.56 3.33 86 CA1 0.76 0.68 0.08 11
N2 4.02 1.02 3.00 75 CA2 N.D. N.D. - -
N3 4.89 N.D. 4.80 98 CA3 N.D. N.D. - -
N4 9.17 0.08 8.92 99 CA4 N.D. N.D. - -
•Normal – ADH Inhibition with 4-MP ranges from 75-99%
•Cancer – Only one sample showed any uninhibited ADH activity followed by 11% inhibition with addition of 4-MP.
Normal Tissue Normal Tissue ImmunocytochemistryImmunocytochemistry
Note organized ducts and Note organized ducts and strong ADH I stainingstrong ADH I staining
Normal ductal epithelium - showing Normal ductal epithelium - showing high immunoreactivity with minimally high immunoreactivity with minimally
reactive stromal cells highlightedreactive stromal cells highlighted
Bar = 5 µm
Normal DuctNormal Duct
Bar = 10µm
Type 3 lobules, parous Type 3 lobules, parous tissuetissue
Bar = 10µm
TDLUTDLU
Bar = 10 µm
Normal 2Normal 2o o Ab controlAb control
Bar = 10 µm
Malignant Tissue Malignant Tissue ImmunocytochemistryImmunocytochemistry
Note loss of immunoreactivity Note loss of immunoreactivity and lack of proper ductal and lack of proper ductal
orientationorientation
Loss of ADH I stainingLoss of ADH I staining
Bar = 10 µm
Cancer – Minimal ADH I Cancer – Minimal ADH I immunoreactivity immunoreactivity
Bar = 10µm
Weak positive cells surrounding Weak positive cells surrounding areas of no ADH I immunoreactive areas of no ADH I immunoreactive
cellscells
Bar = 10 µm
Increased magnification of Increased magnification of previous slideprevious slide
Bar = 2 µm
Increased MagnificationIncreased Magnification20x vs 100x 20x vs 100x
Bar = 10 µm
Bar = 2 µm
Overall heterogeneity of ADH I Overall heterogeneity of ADH I immunoreactivity immunoreactivity
Bar = 10 µm
Weak ADH I immunoreactivity Weak ADH I immunoreactivity seen in a morphologically seen in a morphologically
“normal” duct“normal” duct
Bar = 5µm
Cancerous tissue – note ducts Cancerous tissue – note ducts lacking expression lacking expression
10x and 40x10x and 40x
Bar = 5 µmBar = 20 µm
Increased magnification Increased magnification 100x100x
Bar = 2 µm
Normal vs. CancerNormal vs. Cancer20x20x
Bar = 10 µm
ReferencesReferencesChambon, P. (1996). A decade of molecular biology of retinoic acid receptors. FASEB. J. 10:940-954.
Duester, G. (1996). Involvement of alcohol dehydrogenase, short-chain dehydrogenase/reductase, aldehyde dehydrogenase, and cytochrome p450 in the control of retinoid signaling by activation of retinoic acid synthesis. Biochemistry. 35, 12221-12227.
Hurley, T., Bosron, W., Stone, C., and L. Amzel. (1997). Structure of three human beta alcohol dehydrogenase variants. J. Mol. Biol. 239:415-429.
Manglesdorf, D., Thummel, C., Beato, M., Herrlich, P., Schutz, G., Umesono, K., Blumberg, B., Kastner, P., Mark, M., Chambon, P., and R. Evans. (1995). The nuclear receptor superfamily: The second decade. Cell. 83:835-839.
Svensson, JBC 274:29712.
Questions?Questions?
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