CB was discovered as a pleomorphic, multi-lamellar, electron-dense, quasi-crystalline stack of condensed and degenerated mitochondrial membranes in the developing UN rat Purkinje neuronal dendrites, hippocampal neural progenitor cells, and in the cardiac progenitor cells (derived from pluripotent stem cells) in response to the environmental neurotoxins, Kainic acid and Domoic acid. CB appears as a nonfunctional intracellular inclusion and is phagocytosed by the lysosomes through ATP-driven CP to sustain ICD. The lysosomes are involved in cell surveillance for maintaining intracellular homeostasis and NCF. CB formation and hence, CP induction, occur frequently due to the structural and functional vulnerability of mitochondrial membranes to free radical-induced lipid peroxidation (as these are highly rich in PUFA) and genetic and epigenetic vulnerability of mtDNA (as it is GC-rich and easily oxidized to form 8-OH, 2dG and methylated at the cytosine residues) as compared to nDNA which is double helical, condensed, and remains protected by histones and protamines. Hence, CP can be utilized as the most sensitive immediate and early biomarker of CB-ATG in any physico-chemically-injured cell. Other organelles including nucleus, lysosomes, peroxisomes, proteasome, and Golgi body, are not phagocytosed as frequently and are spared from the immediate, early, and direct attack of free radicals. The mtDNA is intron-less and remains in a hostile microenvironment of free radicals generated as a byproduct of O/P in the mitochondrial matrix. Moreover, mtDNA is naked, non-helical, devoid of histones and protamines, which render it highly susceptible to genetic and epigenetic modifications. The cytosine is readily methylated by S-adenosyl methionine (SAM) at position N-3 on the naked mtDNA to trigger CBMP. Hence, early detection of 2, 3 dihydroxy nonenal, 4-OH, nonenal and 8-OH, 2dG from the biological fluids can provide a quantitative estimate of mitochondrial bioenergetics (MB) of a patient. On the other hand, the nDNA is supercoiled, double helical, compact, and remains protected by the nuclear wall and nucleoplasm. Histones, protamines, and topoisomerases provide structural and functional stability to gyrases to maintain its helicity. Hence, genetic and epigenetic changes occur rarely in the nDNA because histone acetylation at the lysine moieties has to occur first to open the super helical structure to expose the cytosine residues for their methylation.

CBMP is involved in almost all cell possessing mitochondria. As CB is a nonfunctional mitochondrial inclusion, it is phagocytosed upon ubiquitination by ATP-driven lysosomal activation. CP is the most sensitive, immediate and early event of CMB to form a CPS. The CPS is transformed to CS, when the phagocytosed CB is hydrolyzed by the lysosomal enzymes. Secondary free radical attack (SFA) causes CS destabilization.

In vivo as well as in vitro experimental data suggest that mitochondria in the most vulnerable cell exhibit differential susceptibility to free radical-induced CBMP in response to endogenous or exogenous DPCI. Depending on the metabolic and physiological needs, a cell may possess anywhere between 22-1000 mitochondria. For example, a sperm has 22-75 spirally-arranged compact mitochondria in the middle piece for motility and fertilization, whereas a neuron may have between 750-1000 mitochondria (Purkinje neurons). Terminally differentiated cells (including skeletal muscle, cardiac, hepatocytes, osteocytes, and CNS neurons) have a fixed number of mitochondria. An oocyte has the maximum mitochondria (250,000-600,000) because it needs sufficient energy to execute paternal CP as well as CS exocytosis during the pre-zygotic phase soon after fertilization, and during the development of the embryo in the post-zygotic phase for the normal growth of the fetus. Osteoblasts also possess a high number of mitochondria for osteogenesis. About 40% of the myocardial and skeletal muscles, 20% of the liver tissue, and 15% of the CNS is composed exclusively of mitochondria as these are metabolically high-energy-demanding tissues. Although, it depends primarily on the frequency and intensity of free radical attack, all mitochondria are not destroyed at any given time in response to DPCI. The exact molecular mechanism of differential and selective vulnerability of mitochondria to free radical-induced CBMP remains enigmatic.

Although both CP and ATG require (i) Akt-ubiquitination of nonfunctional organelles and associated proteins in response to DPCI-induced free radical attack on the most vulnerable stem cell and ATP-driven lysosomal activation, CP involves predominantly phagocytosis of CB during mitochondrial remodeling (MR) and degeneration. Generally, ATG is nonspecific and can phagocytose any nonfunctional, degenerated, and/or undesired intracellular organelle. CP can selectively influence cell death, inflammation, immune response, and exert both adaptive and maladaptive roles in disease pathogenesis. CBMP involving CB formation, CP induction, and CS destabilization are deleterious events as these are implicated in chronic MDR diseases. Although, increased lysosomal activity triggers pro-inflammatory cascade in a physicochemical-injured cell during the acute phase; enhanced CP increases the incidence of CS destabilization which triggers inflammasome to cause MDR diseases during chronic phase. Hence, CP-mediated CB elimination is highly prudent to sustain IMD and ICD for NCF.