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  • Title
  • DECLARATION
  • CERTIFICATE
  • ACKNOWLEDGEMENT
  • CONTENTS
  • ABBREVIATIONS
  • 1 Introduction
  • 1.1 PLANTS AND HEALTH CARE
  • 1.2 Cancer
  • 1.2.1 Cancer Treatment Modalities
  • 1.3 Development of a drug for cancer
  • 1.3.1 Development of anticancer drugs from plants
  • 1.3.2 Bioassays of plant products
  • 1.4 Plants used in the treatment of Cancer
  • 1.4.1 Cytotoxic and antitumour principles
  • 1.5 Apoptosis
  • 1.5.1 BCL2 family: Killers and protectors
  • 1.5.1 Therapeutic implications
  • 1.6 Chromosomes
  • 1.7.1 Modulators of the toxicity of the anticancer drugs vincristine and cyclophosphamide
  • 1.8 Infrared Spectroscopy
  • 1.8.1 Spectroscopy of major cellular components
  • 1.8.2 Infrared Absorption Spectra of Protein and Nucleic acids
  • 1.9 Rationale for the selection of the plant of this study
  • 1.9.1 Properties and Uses of B.racemosa seed
  • 1.9.2 Chemistry and Pharmacology
  • 1.I0 Aims and Objectives
  • 2 MATERIALS AND METHODS
  • 2.1 MATERIALS
  • 2.1.1 Plants
  • 2.1.2 Experimental animals
  • 2.1.3 Tumour Cell Lines
  • 2.1.4 Chemicals
  • 2.1.5 Instruments
  • 2.2 METHODS
  • 2.2.1 Methods for separation and purification of phytochemicals
  • 2.2.2 Extraction and Purification of B.racemosa seeds
  • 2.2.2.1 B.racemosa seed extract
  • 2.2.2.2 Purification of the methanol extract of B.racemosa seed extract
  • 2.3 Toxicity studies
  • 2.3.1 Acute toxicity
  • 2.3.2 Short-term toxicity
  • 2.4 Assessment of anticancer activity
  • 2.4.1 Experimental Animal Maintenance
  • 2.4.2 Maintenance of tumour cell lines in mice
  • 2.5 Tissue Culture
  • 2.5.1 Determination of cytotoxicity using cell culture
  • 2.5.2 Short-term Cytotoxicity
  • 2.6 Anti tumour testing using murine models
  • 2.7 Determination of Apoptosis
  • 2.7.1 in vitro study
  • 2.7.2 in vivostudy
  • 2.8 Chromosomal aberration studies
  • 2.9 Modulation of the toxicity induced by the antiturnour drugscyclophosphamide and vincristine
  • 2.9.1 Modulation of Vincristine induced toxicities in normal mice
  • 2.9.2 Modulation of toxicities in tumour bearing mice treatedVincristine
  • 2.9.3 Modulation of cyclophosphamide induced toxicities in normalmice
  • 2.9.4 Modulation of toxicities in tumour bearing mice treated withCyclophosphamide
  • 2.9.5 Haematological parameters
  • 2.9.5.1 Method
  • 2.9.5.2 Red and White cell counting
  • 2.9.5.3 Platelets count and size distribution
  • 2.9.5.4 Measurement of hemoglobin concentration
  • 2.9.5.5 Derivation of parameters
  • 2.9.5.6 Determination of serum alkaline phosphatase
  • 2.9.5.7 Determination of SGPT
  • 2.5.9.8 Determination of SGOT
  • 2.5.9.9 Determination of Urea
  • 2.5.9.10 Quantitative determination of inorganic phosphate in serum
  • 2.5.9.11 Estimation of calcium [0- cresolphthalein Complexone Method]
  • 2.6 IR Spectroscopy
  • 2.6.1 Mice
  • 2.6.2 Preparation of cell lines
  • 2.6.3 Solid tumour growth formation
  • 2.6.4 Histopathological studies
  • 2.7 Statistical analysis
  • 3 CYTOTOXICITY TO TUMOUR CELLS AND CELLS IN CULTURE (IN VITRO)
  • 3.1 introduction
  • 3.2 Materials and Methods
  • 3.2.1 Preparation of seed extract
  • 3.2.2 Purification of the seed extract
  • 3.2.4 Toxicity
  • 3.2.4.1 Acute toxicity
  • 3.2.4.2 Short-term toxicity
  • 3.3 In vitro cytotoxicity
  • 3.3.1 Ascitic tumour cells
  • 3.3.2 In vitro cell culture
  • 3.5 Results
  • 3.5.1 Toxicity
  • 3.6 Discussion
  • 4 ANTI -TUMOUR ACTNITY STUDIES
  • 4.1 INTRODUCTION
  • 4.2 Materials and Methods
  • 4.2.1 Antiturnour testing using rnurine models
  • 4.2.2 Effect of methanol extract of B.racemosa seed on the growth of ascitic tumour in mice
  • 4.2.3 Treatment Schedule
  • 4.2.4 Effect of purified fractions F5 (7: 3) and F8 (2: 8) of B.racemosa seed extract on the growth of ascitic tumours in mice.
  • 4.2.5 Effect of the drug on solid tumour in mice
  • 4.3 Results
  • 4.3.1 Effect of the drug (s) on the growth of solid tumour
  • 4.4 Discussion
  • 5 THE EFFECT OF THE DRUG ON APOPTOSIS
  • 5.1 INTRODUCTION
  • 5.2 Biochemistry of apoptosis
  • 5.3 Apoptosis induced by Medicinal plants
  • 5.4 Materials and Methods
  • 5.4.1 Mice:
  • 5.4.2 DLA Cell-line:
  • 5.4.3 Purification of B.racemosa seed extract:
  • 5.4.4 lnvitro study:
  • 5.4.5 Invivo study:
  • 5.4.6 Morphologic determination of apoptosis
  • 5.5 Result
  • 5.6 Discussion
  • 6 ANTI -CLASTOGENIC ACTIVITY OFBARRINGTONIA RACEMOSA SEED EXTRACT
  • 6.1 INTRODUCTION
  • 6.2 Materials and Methods
  • 6.3 Slide preparation and chromosome aberration scoring
  • 6.4 Results
  • 6.5 Discussion
  • 7 MODULATION OF TOXICITY OF THE ANTI-CANCER DRUGS, VINCRISTINEAND CYCLOPHOSPHMIDE
  • 7.1 INTRODUCTION
  • 7.2 Materials and Methods
  • 7.2.1 Mice
  • 7.2.2 Drugs
  • 7.2.3 Cyclophosphamide treated normal mice
  • 7.2.4 Cyclophosphamide treated tumour bearing mice
  • 7.2.5 Vincristine treated normal mice
  • 7.2.6 Vincristine treated tumour bearing mice
  • 7.2.7 Haematological and biochemical parameters
  • 7.3 Result
  • 7.3.1 Cyclophosphamide treated normal mice
  • 7.3.2 CYP treated tumour bearing mice
  • 7.3.3 Vincristine treated normal mice
  • 7.3.4 Vincristine treated tumour bearing mice
  • 7.4 Discussion
  • 8 INFRARED SPECTROSCOPIC STUDIES OF NORMAL DLA INDUCED TUMOUR AND DRUG TREATED TUMOUR
  • 8.1 INTRODUCTION
  • 8.2 Materials and Methods
  • 8.2.1 Mice:
  • 8.2.2 Preparation of cell lines
  • 8.2.3 Solid tumour growth formation
  • 8.2.4 Infrared Spectroscopic Analysis of DLA induced tumour tissue, drug treated tumour and control (normal thy muscle)
  • 8.2.5 Histopathological studies
  • 8.3 Results
  • 8.3.1 Inhibition of solid tumour growth
  • 8.3.2 IR spectroscopic studies
  • 8.3.3 Histopathological studies
  • 8.4 Discussion
  • 9 GENERAL DISCUSSION
  • 9.1 GENERAL DISCUSSION
  • SUMMARY AND CONCLUSIONS
  • REFERENCES
  • LIST OF PUBLICATIONS
  • ABSTRACT