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Dr Davis Nadakkavukaran.M.D.S
SENIOR LECTURER
MALABAR DENTAL COLLEGE
MANOOOR
 Introduction
 Aims of staging
 Method of staging
 Stage grouping
 Limitations of staging
 Types of Biomarkers
 Commonly used biomarkers
 Conclusion
 References
 (a) cancer cells are derived from the body’s own cells
 (b) cancer cells generally continue to grow in an
unlimited fashion, at least when they have reached a
size that leads to their being diagnosed
 (c) they often infiltrate, i.e. they grow into and destroy
the surrounding normal tissue
 (d) they can spread via blood and/or lymphatic vessels
and cause secondary growths- known as metastases-
in other organs.
In general, malignant neoplasms in humans and
rodents develop through multistep processes During
such processes, several genetic alterations occur
 The tumor-node-metastasis (TNM) staging system was first
reported by Pierre Denoix in the 1940.
 The International Union Against Cancer (UICC) eventually
adapted the system and compiled the first edition of the TNM
staging system in 1968 for 23 body sites.
 TNM staging system is simply an anatomic staging system
that describes the anatomic extent of the primary tumor as
well as the involvement of regional lymph nodes and distant
metastasis
 The overwhelming majority of mucosal HNCs are squamous
cell carcinomas. Therefore, the TNM classification of the UICC
and the American Joint Committee on Cancer (AJCC) for most
mucosal anatomic sites is designed for squamous cell
carcinoma and minor salivary gland cancers.
 Why staging?
 An aid to planning therapy
 Indication of prognosis
Comparison of results of treatment
Facilitate exchange of information between
treatment centres
Statistics and trends
 T –Extent of primary tumour
 N –Presence or absence and extent of
nodal involvement
 M –Presence or absence of distant
metastasis
 Clinical classification designated as cTNM
or TNM
Pathological classification designated
pTNM
 Retreatment classification designated
rTNM
 Autopsy designated aTNM
STAGIN
G
T
M
N
STAGIN
G
T
M
N
STAGIN
G
T
M
N
Limitation of T Staging
 crude system
 Tumour size not consistently related to
prognosis
Debatable anatomic boundaries
Can be difficult to accurately assess
clinical extent
 Inconsistencies
 Omissions
Observer variability ( presence of nodal
disease and size measurement)
No inclusion of immunological status
Importance of extracapsular spread
N2 (bilateral involvement ) implies better
prognosis than N3 (large nodes greater
than 6 cm
 The histologic grade is a qualitative
assessment of the differentiation of the
tumour expressed as the extent as to which a
tumour resembles the normal tissue at that
site
 GX Grade cannot be assessed
 G1Well differentiated
 G2Moderately differentiated
 G3 Poorly differentiated
 G4Undifferentiated
 The National Cancer Institute (NCI), in
particular, defines biomarker as a:
 “A biological molecule found in blood, other
body fluids, or tissues that is a sign of a
normal or abnormal process, or of a condition
or disease.
 A biomarker maybe used to see how well the
body responds to a treatment for a disease or
condition. Also called molecular marker and
signature molecule."
 Screening in general population
 Differential diagnosis in symptomatic patients
 Clinical staging of cancer
 Estimating tumour volume
 Prognostic indicator for disease progression
 Detecting recurrences
 Monitoring responses to therapy
 Radioimmuno localization of tumour masses
 Determining direction for immunotherapy
 It should have high sensitivity and specificity.
 It should have high positive and negative predictive
value.
 It should be able to differentiate between neoplastic
and non-neoplastic disease and show positive
correlation with tumor volume and extent
 It should predict early recurrence and have prognostic
value
 It should be clinically sensitive, i.e. detectable at early
stage of tumor
 Its levels should be preceding the neoplastic process,
so can be useful for screening
 It should be easily assayable
• ELISA
• Immuno-histochemistry (IHC)
• Polymerase chain reaction (PCR)
• Fluorescence in situ hybridization (FISH)
• Cluster Kits ( All-in-One Kit)
– Detects profiles
– Patterns
– Prototypes
– Constellations
(a) Epithelial markers
Cell surface markers –Histocompatibility
Intracellular markers –Cytokeratins
Basement membrane markers –Type 4
collagen
Matrix markers –Tenascin
Membrane antigen –Blood group antigens.
(b) Connective tissue markers
Intermediate filament proteins –Desmin
Other filament proteins –Laminin
Cellular enzymes –Amylase, lysozyme
Cytoplasmic non-filamentous
non-enzymatic proteins –Myoglobin, S100
protein
Membrane antigen –Leukocyte specific
antigen.
(c) Salivary gland marker
Myoepithelial cell markers –Actin, myosin
Serum acinar cell markers –Salivary
amylase
Myoepithelial cells + acinar cells –S100
protein.
Serum tumour markers
Oncofetal proteins (Alpha fetoprotein,
Carcinoembryonic antigen)
B Protein
Enzymes (LDH)
Beta 2 microglobulin
 This is significantly increased in OSCC
patients
Direct correlation with increasing staging
and nodal status
 Measured with ELISA
 Can be used as a good tool for prognosis
Ecological and observational studies
suggest that low serum albuminis
associated with higher mortality from
cancer.
 Pre treatment serum albumin levels can
provide useful prognostic information in a
variety of cancers
 Enzyme is found in the cells of almost all body
tissues
 Anerobic condition:
PYRUVATE
LACTIC ACID
 Increased LDH levels are due to increased
mitotic index and more lactic acid production by
tumor cells due to breakdown of glycoprotein
 increased levels of serum LDH in patients with
OSCC and the levels correlated positively with
the clinical stage of the disease
LDH
 Tumor proteins may induce the formation of
autoantibodies which can be detected in patient
serum.
 Separate protein lysates from human SCC cell
lines, followed by Western Blotting using patient
sera.
 Antigens are then identified using mass
spectrometry
 Eg: Heat shock protein 70, sideroflexin 3
 It has been suggested that these autoantibodies
might be used to establish effective new immune
therapies, besides using them for early diagnosis
of these tumors.
 Antioxidant enzymes such as superoxide
dismutase and catalase can directly counter
balance the oxidant attack and may protect cells
against DNA damage.
 Studies have shown that erythrocyte superoxide
dismutase activity was decreased in oral cancer
patients than in healthy individuals and patients
with oral lichen planus (OLP).
 The low activity of erythrocyte superoxide
dismutase can be due to the depletion of
antioxidant defense system, occurring as a
consequence of overwhelming free radicals.
 Keratins as tumor markers have two main applications:
 In distinguishing epithelial from non-epithelial tumors
 In distinguishing the type of epithelial tumor
 The most obvious example is IL-1β whose values in saliva
were the highest of all the studied cytokines, while in serum its
values were below the level of detection.
 It is shown that patients with oral cancer have significantly
higher concentrations of salivary IL-1β and IL-6 compared to
patients with leukoplakia and healthy individuals.
 Increase in the concentrations of proinflammatory cytokines in
saliva might reflect the development of oral cancer from oral
leukoplakia.
 Chronic inflammation constitutes one of the key risk factors
for OSCC. Studies indicate that IL-6–induced inflammation
promotes tumorigenesis in the oral cavity by altering global
LINE-1 hypomethylation.
 The CD44 family of receptors includes multiple
variant isoforms, several of which have been linked
to malignant properties including migration,
invasion, and metastasis.
 Expression of CD44 variant isoforms was
associated with advanced T stage (v3 and v6),
regional (v3) and distant (v10) metastasis,
perineural invasion (v6), and radiation failure (v10).
 CD44 v6 and CD44 v10 were also significantly
associated with shorter disease-free survival
 CD59 inhibits the complement membrane attack
complex by binding C5b678 and preventing C9 from
binding and polymerizing. It is present on “self” cells to
prevent complement from damaging them.
 Tumor cells can escape complement-dependent
cytotoxicity (CDC) by expressing complement
restriction factors (CRFs), CD46, CD55, and CD59.
CD46, CD55, and CD59 were highly expressed in
HNSCC cells including T1/T2N0M0 stages.
 The CRF expression was much lower or absent in
non-neoplastic squamous epithelia or in the
submucosa of both normal and tumor tissues.
 IL-8 is an angiogenic chemokine with a
high expression level in the tumor tissues.
This plays important roles in developing
many human malignancies including
OSCC.
 Results suggested that combination of
IL-8 gene polymorphisms and
environmental carcinogens might be highly
related to the risk of oral cancer.
 Endothelins are 21-amino acid
vasoconstricting peptides produced primarily
in the endothelium, and have a key role in
vascular homeostasis.
 Salivary endothelin-1 (ET-1) could be a good
biomarker for OSCC development in OLP
patients regardless of the degree of OLP
disease activity.
 However, it appeared not to be a good
biomarker for detecting recurrence of OSCC
in patients in remission
 also known as 90K, is a highly glycosylated,
secreted protein extensively studied in human
cancer, which binds galectin-1, galectin-3,
and galectin-7.
 High expression levels of 90K are associated
with a shorter survival, the occurrence of
metastasis, or a reduced response to
chemotherapy in patients with different types
of malignancy
 Tissue polypeptide antigen Tissue
polypeptide antigen (TPA), regarded as a
marker of cell proliferation, is a mixture of
fragments containing relatively stable
a-helical rod domains of simple
epithelium-type cytokeratins.
 These fragments are probably released
during necrosis and lysis of the carcinoma
cells. TPA is known to be a sensitive, but
nonspecific tumor marker. Thus, TPA should
be regarded as a broad-spectrum epithelial
tumor marker
 The possible correlation of TNF-a and -b
genes with the risk of oral cancer was
investigated in a study. The functional
polymorphisms TNF-a and TNF-b, which
affect gene expression, were investigated by
restriction fragment length polymorphism
analysis.
 The frequencies of high-expression A2 TNF-a
allele and high expression B1 TNF-b allele
were significantly increased in cancer patients
compared to control.
To evaluate the usefulness of a tumor
marker, it is necessary to
 Find reference values,
calculate predictive values,
evaluate distribution of marker values, and
determine the role of these values in
disease management
 Stell and Maran’s Head and Neck surgery and Oncology
 AJCC cancer staging manual 6th Ed
 Pocket Guide To TNM STAGING OF HEAD AND NECK
CANCER AND NECK DISSECTION CLASSIFICATION
 Bhatt AN, Mathur R, Farooque A,Verma A, Dwarakanath B.S.
Cancer biomarkers - Current perspectives. Indian J Med Res
132, August 2010, pp 129-149
 Cheng et al. A review of research on salivary biomarkers for
oral cancer detectionClinical and Translational Medicine 2014,
3:3
 Choontharu MM, Binda A, Bhat S, Sharma SM. Role of tumor
markers in oral squamous cell carcinoma: Review of literature
and future consideration. SRM J Res Dent Sci 2012;3:251-6

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Staging an tumor markers

  • 1. Dr Davis Nadakkavukaran.M.D.S SENIOR LECTURER MALABAR DENTAL COLLEGE MANOOOR
  • 2.  Introduction  Aims of staging  Method of staging  Stage grouping  Limitations of staging  Types of Biomarkers  Commonly used biomarkers  Conclusion  References
  • 3.  (a) cancer cells are derived from the body’s own cells  (b) cancer cells generally continue to grow in an unlimited fashion, at least when they have reached a size that leads to their being diagnosed  (c) they often infiltrate, i.e. they grow into and destroy the surrounding normal tissue  (d) they can spread via blood and/or lymphatic vessels and cause secondary growths- known as metastases- in other organs. In general, malignant neoplasms in humans and rodents develop through multistep processes During such processes, several genetic alterations occur
  • 4.  The tumor-node-metastasis (TNM) staging system was first reported by Pierre Denoix in the 1940.  The International Union Against Cancer (UICC) eventually adapted the system and compiled the first edition of the TNM staging system in 1968 for 23 body sites.  TNM staging system is simply an anatomic staging system that describes the anatomic extent of the primary tumor as well as the involvement of regional lymph nodes and distant metastasis  The overwhelming majority of mucosal HNCs are squamous cell carcinomas. Therefore, the TNM classification of the UICC and the American Joint Committee on Cancer (AJCC) for most mucosal anatomic sites is designed for squamous cell carcinoma and minor salivary gland cancers.
  • 5.  Why staging?  An aid to planning therapy  Indication of prognosis Comparison of results of treatment Facilitate exchange of information between treatment centres Statistics and trends
  • 6.  T –Extent of primary tumour  N –Presence or absence and extent of nodal involvement  M –Presence or absence of distant metastasis
  • 7.  Clinical classification designated as cTNM or TNM Pathological classification designated pTNM  Retreatment classification designated rTNM  Autopsy designated aTNM
  • 9.
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  • 19.
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  • 23. Limitation of T Staging  crude system  Tumour size not consistently related to prognosis Debatable anatomic boundaries Can be difficult to accurately assess clinical extent  Inconsistencies  Omissions
  • 24. Observer variability ( presence of nodal disease and size measurement) No inclusion of immunological status Importance of extracapsular spread N2 (bilateral involvement ) implies better prognosis than N3 (large nodes greater than 6 cm
  • 25.  The histologic grade is a qualitative assessment of the differentiation of the tumour expressed as the extent as to which a tumour resembles the normal tissue at that site  GX Grade cannot be assessed  G1Well differentiated  G2Moderately differentiated  G3 Poorly differentiated  G4Undifferentiated
  • 26.
  • 27.  The National Cancer Institute (NCI), in particular, defines biomarker as a:  “A biological molecule found in blood, other body fluids, or tissues that is a sign of a normal or abnormal process, or of a condition or disease.  A biomarker maybe used to see how well the body responds to a treatment for a disease or condition. Also called molecular marker and signature molecule."
  • 28.  Screening in general population  Differential diagnosis in symptomatic patients  Clinical staging of cancer  Estimating tumour volume  Prognostic indicator for disease progression  Detecting recurrences  Monitoring responses to therapy  Radioimmuno localization of tumour masses  Determining direction for immunotherapy
  • 29.  It should have high sensitivity and specificity.  It should have high positive and negative predictive value.  It should be able to differentiate between neoplastic and non-neoplastic disease and show positive correlation with tumor volume and extent  It should predict early recurrence and have prognostic value  It should be clinically sensitive, i.e. detectable at early stage of tumor  Its levels should be preceding the neoplastic process, so can be useful for screening  It should be easily assayable
  • 30. • ELISA • Immuno-histochemistry (IHC) • Polymerase chain reaction (PCR) • Fluorescence in situ hybridization (FISH) • Cluster Kits ( All-in-One Kit) – Detects profiles – Patterns – Prototypes – Constellations
  • 31. (a) Epithelial markers Cell surface markers –Histocompatibility Intracellular markers –Cytokeratins Basement membrane markers –Type 4 collagen Matrix markers –Tenascin Membrane antigen –Blood group antigens.
  • 32. (b) Connective tissue markers Intermediate filament proteins –Desmin Other filament proteins –Laminin Cellular enzymes –Amylase, lysozyme Cytoplasmic non-filamentous non-enzymatic proteins –Myoglobin, S100 protein Membrane antigen –Leukocyte specific antigen.
  • 33. (c) Salivary gland marker Myoepithelial cell markers –Actin, myosin Serum acinar cell markers –Salivary amylase Myoepithelial cells + acinar cells –S100 protein.
  • 34. Serum tumour markers Oncofetal proteins (Alpha fetoprotein, Carcinoembryonic antigen) B Protein Enzymes (LDH) Beta 2 microglobulin
  • 35.  This is significantly increased in OSCC patients Direct correlation with increasing staging and nodal status  Measured with ELISA  Can be used as a good tool for prognosis
  • 36. Ecological and observational studies suggest that low serum albuminis associated with higher mortality from cancer.  Pre treatment serum albumin levels can provide useful prognostic information in a variety of cancers
  • 37.  Enzyme is found in the cells of almost all body tissues  Anerobic condition: PYRUVATE LACTIC ACID  Increased LDH levels are due to increased mitotic index and more lactic acid production by tumor cells due to breakdown of glycoprotein  increased levels of serum LDH in patients with OSCC and the levels correlated positively with the clinical stage of the disease LDH
  • 38.  Tumor proteins may induce the formation of autoantibodies which can be detected in patient serum.  Separate protein lysates from human SCC cell lines, followed by Western Blotting using patient sera.  Antigens are then identified using mass spectrometry  Eg: Heat shock protein 70, sideroflexin 3  It has been suggested that these autoantibodies might be used to establish effective new immune therapies, besides using them for early diagnosis of these tumors.
  • 39.  Antioxidant enzymes such as superoxide dismutase and catalase can directly counter balance the oxidant attack and may protect cells against DNA damage.  Studies have shown that erythrocyte superoxide dismutase activity was decreased in oral cancer patients than in healthy individuals and patients with oral lichen planus (OLP).  The low activity of erythrocyte superoxide dismutase can be due to the depletion of antioxidant defense system, occurring as a consequence of overwhelming free radicals.
  • 40.  Keratins as tumor markers have two main applications:  In distinguishing epithelial from non-epithelial tumors  In distinguishing the type of epithelial tumor  The most obvious example is IL-1β whose values in saliva were the highest of all the studied cytokines, while in serum its values were below the level of detection.  It is shown that patients with oral cancer have significantly higher concentrations of salivary IL-1β and IL-6 compared to patients with leukoplakia and healthy individuals.  Increase in the concentrations of proinflammatory cytokines in saliva might reflect the development of oral cancer from oral leukoplakia.  Chronic inflammation constitutes one of the key risk factors for OSCC. Studies indicate that IL-6–induced inflammation promotes tumorigenesis in the oral cavity by altering global LINE-1 hypomethylation.
  • 41.  The CD44 family of receptors includes multiple variant isoforms, several of which have been linked to malignant properties including migration, invasion, and metastasis.  Expression of CD44 variant isoforms was associated with advanced T stage (v3 and v6), regional (v3) and distant (v10) metastasis, perineural invasion (v6), and radiation failure (v10).  CD44 v6 and CD44 v10 were also significantly associated with shorter disease-free survival
  • 42.  CD59 inhibits the complement membrane attack complex by binding C5b678 and preventing C9 from binding and polymerizing. It is present on “self” cells to prevent complement from damaging them.  Tumor cells can escape complement-dependent cytotoxicity (CDC) by expressing complement restriction factors (CRFs), CD46, CD55, and CD59. CD46, CD55, and CD59 were highly expressed in HNSCC cells including T1/T2N0M0 stages.  The CRF expression was much lower or absent in non-neoplastic squamous epithelia or in the submucosa of both normal and tumor tissues.
  • 43.  IL-8 is an angiogenic chemokine with a high expression level in the tumor tissues. This plays important roles in developing many human malignancies including OSCC.  Results suggested that combination of IL-8 gene polymorphisms and environmental carcinogens might be highly related to the risk of oral cancer.
  • 44.  Endothelins are 21-amino acid vasoconstricting peptides produced primarily in the endothelium, and have a key role in vascular homeostasis.  Salivary endothelin-1 (ET-1) could be a good biomarker for OSCC development in OLP patients regardless of the degree of OLP disease activity.  However, it appeared not to be a good biomarker for detecting recurrence of OSCC in patients in remission
  • 45.  also known as 90K, is a highly glycosylated, secreted protein extensively studied in human cancer, which binds galectin-1, galectin-3, and galectin-7.  High expression levels of 90K are associated with a shorter survival, the occurrence of metastasis, or a reduced response to chemotherapy in patients with different types of malignancy
  • 46.  Tissue polypeptide antigen Tissue polypeptide antigen (TPA), regarded as a marker of cell proliferation, is a mixture of fragments containing relatively stable a-helical rod domains of simple epithelium-type cytokeratins.  These fragments are probably released during necrosis and lysis of the carcinoma cells. TPA is known to be a sensitive, but nonspecific tumor marker. Thus, TPA should be regarded as a broad-spectrum epithelial tumor marker
  • 47.  The possible correlation of TNF-a and -b genes with the risk of oral cancer was investigated in a study. The functional polymorphisms TNF-a and TNF-b, which affect gene expression, were investigated by restriction fragment length polymorphism analysis.  The frequencies of high-expression A2 TNF-a allele and high expression B1 TNF-b allele were significantly increased in cancer patients compared to control.
  • 48. To evaluate the usefulness of a tumor marker, it is necessary to  Find reference values, calculate predictive values, evaluate distribution of marker values, and determine the role of these values in disease management
  • 49.
  • 50.  Stell and Maran’s Head and Neck surgery and Oncology  AJCC cancer staging manual 6th Ed  Pocket Guide To TNM STAGING OF HEAD AND NECK CANCER AND NECK DISSECTION CLASSIFICATION  Bhatt AN, Mathur R, Farooque A,Verma A, Dwarakanath B.S. Cancer biomarkers - Current perspectives. Indian J Med Res 132, August 2010, pp 129-149  Cheng et al. A review of research on salivary biomarkers for oral cancer detectionClinical and Translational Medicine 2014, 3:3  Choontharu MM, Binda A, Bhat S, Sharma SM. Role of tumor markers in oral squamous cell carcinoma: Review of literature and future consideration. SRM J Res Dent Sci 2012;3:251-6

Editor's Notes

  1. CANCER, a malignant epithelial neoplasm, is a collective term for at least a hundred different diseases. These can be quite unique from the point of view of cause, histologic appearances, symptoms and prognosis. However, several common characteristic scan be seen: Oral cancer is on the rise in our country and is one of the deadly cancers. The main causative factors are tobacco and alcohol
  2. Tumor markers can be broadly classified based on the type of tissue as follows:
  3. Increased serum LDH activity is considered as a marker of cellular necrosis, and serum LDH