Gene structure is the organisation of specialised sequence elements within a gene. Genes contain most of the information necessary for living cells to survive and reproduce. In most organisms, genes are made of DNA, where the particular DNA sequence determines the function of the gene. A gene is transcribed (copied) from DNA into RNA, which can either be non-coding RNA (ncRNA) with a direct function, or an intermediate messenger RNA (mRNA) that is then translated into protein.
Each of these steps is controlled by specific sequence elements, or
regions, within the gene. Every gene, therefore, requires multiple
sequence elements to be functional. This includes the sequence that actually encodes the functional protein or ncRNA, as well as multiple regulatory sequence regions. These regions may be as short as a few base pairs, up to many thousands of base pairs long.
Much of gene structure is broadly similar between eukaryotes and prokaryotes. These common elements largely result from the shared ancestry of cellular life in organisms over 2 billion years ago. Key differences in gene structure between eukaryotes and prokaryotes
reflect their divergent transcription and translation machinery. Understanding gene structure is the foundation of understanding gene annotation, expression, and function.
Common features
The
structures of both eukaryotic and prokaryotic genes involve several
nested sequence elements. Each element has a specific function in the
multi-step process of gene expression. The sequences and lengths of these elements vary, but the same general functions are present in most genes. Although DNA is a double-stranded molecule, typically only one of the strands encodes information that the RNA polymerase reads to produce protein-coding mRNA or non-coding RNA. This 'sense' or 'coding' strand, runs in the 5' to 3' direction where the numbers refer to the carbon atoms of the backbone's ribose sugar. The open reading frame (ORF) of a gene is therefore usually represented as an arrow indicating the direction in which the sense strand is read.
Regulatory sequences are located at the extremities of genes. These sequence regions can either be next to the transcribed region (the promoter) or separated by many kilobases (enhancers and silencers). The promoter is located at the 5' end of the gene and is composed of a
core promoter sequence and a proximal promoter sequence. The core
promoter marks the start site for transcription by binding RNA
polymerase and other proteins necessary for copying DNA to RNA. The
proximal promoter region binds transcription factors that modify the affinity of the core promoter for RNA polymerase. Genes may be regulated by multiple enhancer and silencer sequences that further modify the activity of promoters by binding activator or repressor proteins. Enhancers and silencers may be distantly located from the gene, many
thousands of base pairs away. The binding of different transcription
factors, therefore, regulates the rate of transcription initiation at
different times and in different cells.
Regulatory elements can overlap one another, with a section of
DNA able to interact with many competing activators and repressors as
well as RNA polymerase. For example, some repressor proteins can bind to
the core promoter to prevent polymerase binding. For genes with multiple regulatory sequences, the rate of transcription is the product of all of the elements combined. Binding of activators and repressors to multiple regulatory sequences has a cooperative effect on transcription initiation.
Although all organisms use both transcriptional activators and
repressors, eukaryotic genes are said to be 'default off', whereas
prokaryotic genes are 'default on'. The core promoter of eukaryotic genes typically requires additional
activation by promoter elements for expression to occur. The core
promoter of prokaryotic genes, conversely, is sufficient for strong
expression and is regulated by repressors.
An additional layer of regulation occurs for protein coding genes
after the mRNA has been processed to prepare it for translation to
protein. Only the region between the start and stop codons encodes the final protein product. The flanking untranslated regions (UTRs) contain further regulatory sequences. The 3' UTR contains a terminator sequence, which marks the endpoint for transcription and releases the RNA polymerase. The 5’ UTR binds the ribosome, which translates the protein-coding region into a string of amino acids that fold to form the final protein product. In the case of genes for non-coding RNAs, the RNA is not translated but instead folds to be directly functional.
Eukaryotes
The structure of eukaryotic genes includes features not found in prokaryotes. Most of these relate to post-transcriptional modification of pre-mRNAs to produce mature mRNA
ready for translation into protein. Eukaryotic genes typically have
more regulatory elements to control gene expression compared to
prokaryotes. This is particularly true in multicellular eukaryotes, humans for example, where gene expression varies widely among different tissues.
A key feature of the structure of eukaryotic genes is that their transcripts are typically subdivided into exon and intron regions. Exon regions are retained in the final mature mRNA molecule, while intron regions are spliced out (excised) during post-transcriptional processing. Indeed, the intron regions of a gene can be considerably longer than
the exon regions. Once spliced together, the exons form a single
continuous protein-coding regions, and the splice boundaries are not
detectable. Eukaryotic post-transcriptional processing also adds a 5' cap to the start of the mRNA and a poly-adenosine tail to the end of the mRNA. These additions stabilise the mRNA and direct its transport from the nucleus to the cytoplasm, although neither of these features are directly encoded in the structure of a gene.
The overall organisation of prokaryotic genes is markedly different
from that of the eukaryotes. The most obvious difference is that
prokaryotic ORFs are often grouped into a polycistronic operon
under the control of a shared set of regulatory sequences. These ORFs
are all transcribed onto the same mRNA and so are co-regulated and often
serve related functions. Each ORF typically has its own ribosome binding site
(RBS) so that ribosomes simultaneously translate ORFs on the same mRNA.
Some operons also display translational coupling, where the translation
rates of multiple ORFs within an operon are linked. This can occur when the ribosome remains attached at the end of an ORF
and simply translocates along to the next without the need for a new
RBS. Translational coupling is also observed when translation of an ORF
affects the accessibility of the next RBS through changes in RNA
secondary structure. Having multiple ORFs on a single mRNA is only possible in prokaryotes
because their transcription and translation take place at the same time
and in the same subcellular location.
The operator
sequence next to the promoter is the main regulatory element in
prokaryotes. Repressor proteins bound to the operator sequence
physically obstructs the RNA polymerase enzyme, preventing
transcription. Riboswitches
are another important regulatory sequence commonly present in
prokaryotic UTRs. These sequences switch between alternative secondary
structures in the RNA depending on the concentration of key metabolites.
The secondary structures then either block or reveal important sequence
regions such as RBSs. Introns are extremely rare in prokaryotes and
therefore do not play a significant role in prokaryotic gene regulation.
The morphogenetic field of pattern formation and maintenance during an organism's lifespan
Developmental bioelectricity is the regulation of cell, tissue, and organ-level patterning and behavior by electrical signals during the development of embryonic animals and plants. The charge carrier in developmental bioelectricity is the ion (a charged atom) rather than the electron,
and an electric current and field is generated whenever a net ion flux
occurs. Cells and tissues of all types use flows of ions to communicate
electrically. Endogenous electric currents and fields, ion fluxes, and differences in resting potential across tissues comprise a signalling system. It functions along with biochemical factors, transcriptional networks, and other physical forces to regulate cell behaviour and large-scale patterning in processes such as embryogenesis, regeneration, and cancer suppression.
Overview
Developmental bioelectricity is a sub-discipline of biology, related to, but distinct from, neurophysiology and bioelectromagnetics.
Developmental bioelectricity refers to the endogenous ion fluxes,
transmembrane and transepithelial voltage gradients, and electric
currents and fields produced and sustained in living cells and tissues. This electrical activity is often used during embryogenesis,
regeneration, and cancer suppression—it is one layer of the complex
field of signals that impinge upon all cells in vivo and regulate
their interactions during pattern formation and maintenance. This is
distinct from neural bioelectricity (classically termed
electrophysiology), which refers to the rapid and transient spiking in
well-recognized excitable cells like neurons and myocytes (muscle cells); and from bioelectromagnetics, which refers to the effects of applied
electromagnetic radiation, and endogenous electromagnetics such as biophoton emission and magnetite.
Membrane potential and transepithelial potential.Electric potential difference across corneal epithelium, and the generation of wound electric fields.Distribution of bioelectric potential in the flank of a frog embryo stained with voltage-sensitive fluorescent dye.
The inside/outside discontinuity at the cell surface enabled by a lipid bilayer
membrane (capacitor) is at the core of bioelectricity. The plasma
membrane was an indispensable structure for the origin and evolution of
life itself. It provided compartmentalization permitting the setting of a
differential voltage/potential gradient (battery or voltage source)
across the membrane, probably allowing early and rudimentary bioenergetics that fueled cell mechanisms. During evolution, the initially purely passive diffusion of ions
(charge carriers), become gradually controlled by the acquisition of ion channels, pumps,
exchangers, and transporters. These energetically free (resistors or
conductors, passive transport) or expensive (current sources, active
transport) translocators set and fine tune voltage gradients – resting
potentials – that are ubiquitous and essential to life's physiology,
ranging from bioenergetics, motion, sensing, nutrient transport, toxins
clearance, and signaling in homeostatic and disease/injury conditions.
Upon stimuli or barrier breaking (short-circuit) of the membrane, ions
powered by the voltage gradient (electromotive force) diffuse or leak,
respectively, through the cytoplasm and interstitial fluids (conductors), generating measurable electric currents – net ion fluxes – and fields. Some ions (such as calcium) and molecules (such as hydrogen peroxide)
modulate targeted translocators to produce a current or to enhance,
mitigate or even reverse an initial current, being switchers.
Endogenous bioelectric signals are produced in cells by the
cumulative action of ion channels, pumps, and transporters. In
non-excitable cells, the resting potential across the plasma membrane
(Vmem) of individual cells propagate across distances via electrical
synapses known as gap junctions
(conductors), which allow cells to share their resting potential with
neighbors. Aligned and stacked cells (such as in epithelia) generate
transepithelial potentials (such as batteries in series) and electric
fields, which likewise propagate across tissues. Tight junctions
(resistors) efficiently mitigate the paracellular ion diffusion and
leakage, precluding the voltage short circuit. Together, these voltages
and electric fields form rich and dynamic and patterns inside living
bodies that demarcate anatomical features, thus acting like blueprints for gene expression
and morphogenesis in some instances. More than correlations, these
bioelectrical distributions are dynamic, evolving with time and with the
microenvironment and even long-distant conditions to serve as
instructive influences over cell behavior and large-scale patterning
during embryogenesis, regeneration, and cancer suppression. Bioelectric control mechanisms are an important emerging target for advances in regenerative medicine, birth defects, cancer, and synthetic bioengineering.
History
18th century
Developmental bioelectricity began in the 18th century. Several seminal works stimulating muscle contractions using Leyden jars culminated with the publication of classical studies by Luigi Galvani
in 1791 (De viribus electricitatis in motu musculari) and 1794. In
these, Galvani thought to have uncovered intrinsic electric-producing
ability in living tissues or "animal electricity". Alessandro Volta
showed that the frog's leg muscle twitching was due to a static
electricity generator and from dissimilar metals undergoing or
catalyzing electrochemical reactions. Galvani showed, in a 1794 study, twitching without metal electricity by touching the leg muscle with a deviating cut sciatic nerve, definitively demonstrating "animal electricity". Unknowingly, Galvani with this and related experiments discovered the
injury current (ion leakage driven by the intact membrane/epithelial
potential) and injury potential (potential difference between injured
and intact membrane/epithelium). The injury potential was, in fact, the
electrical source behind the leg contraction, as realized in the next
century. Subsequent work ultimately extended this field broadly beyond nerve and
muscle to all cells, from bacteria to non-excitable mammalian cells.
19th century
Building
on earlier studies, further glimpses of developmental bioelectricity
occurred with the discovery of wound-related electric currents and
fields in the 1840s, when the electrophysiologistEmil du Bois-Reymond
reported macroscopic level electrical activities in frog, fish and
human bodies. He recorded minute electric currents in live tissues and
organisms with a then state-of-the-art galvanometer
made of insulated copper wire coils. He unveiled the fast-changing
electricity associated with muscle contraction and nerve excitation –
the action potentials. Du Bois-Reymond also reported in detail less fluctuating electricity at
wounds – injury current and potential – he made to himself.
Some
sample cell types and their resting potentials, revealing that actively
proliferating and plastic cells cluster in the depolarized end of the
continuum, while terminally-differentiated mature cell types tend to be
strongly polarized.
Early 20th century
Developmental bioelectricity work began in earnest at the beginning of the 20th century. Ida H. Hyde studied the role of electricity in the development of eggs. T. H. Morgan and others studied the electrophysiology of the earthworm. Oren E. Frazee studied the effects of electricity on limb regeneration in amphibians. E. J. Lund explored morphogenesis in flowering plants. Libbie Hyman studied vertebrate and invertebrate animals.
In the 1920s and 1930s, Elmer J. Lund and Harold Saxton Burr wrote multiple papers about the role of electricity in embryonic development. Lund measured currents in a large number of living model systems,
correlating them to changes in patterning. In contrast, Burr used a
voltmeter to measure voltage gradients, examining developing embryonic
tissues and tumors, in a range of animals and plants. Applied electric
fields were demonstrated to alter the regeneration of planarian by Marsh and Beams in the 1940s and 1950s, inducing the formation of heads or tails at cut sites, reversing the primary body polarity.
Late 20th century
In
the 1970s, Lionel Jaffe and Richard Nuccittelli's introduction and
development of the vibrating probe, the first device for quantitative
non-invasive characterization of the extracellular minute ion currents,
revitalized the field.
Researchers such as Joseph Vanable, Richard Borgens, Ken
Robinson, and Colin McCaig explored the roles of endogenous bioelectric
signaling in limb development and regeneration, embryogenesis, organ
polarity, and wound healing.
C.D. Cone studied the role of resting potential in regulating cell differentiation and proliferation. Subsequent work has identified specific regions of the resting potential
spectrum that correspond to distinct cell states such as quiescent,
stem, cancer, and terminally differentiated.
Although this body of work generated a significant amount of
high-quality physiological data, this large-scale biophysics approach
has historically come second to the study of biochemical gradients and
genetic networks in biology education, funding, and overall popularity
among biologists. A key factor that contributed to this field lagging
behind molecular genetics and biochemistry is that bioelectricity is
inherently a living phenomenon – it cannot be studied in fixed
specimens. Working with bioelectricity is more complex than traditional
approaches to developmental biology, both methodologically and
conceptually, as it typically requires a highly interdisciplinary
approach.
Study techniques
Electrodes
The
gold standard techniques to quantitatively extract electric dimensions
from living specimens, ranging from cell to organism levels, are the
glass microelectrode (or micropipette), the vibrating (or self-referencing) voltage probe, and the vibrating ion-selective microelectrode. The former is inherently invasive, and the two latter are non-invasive, but all are ultra-sensitive and fast-responsive sensors extensively used in a plethora of physiological conditions in widespread biological models.
The glass microelectrode was developed in the 1940s to study the
action potential of excitable cells, deriving from the seminal work by
Hodgkin and Huxley in the giant axon squid. It is simply a liquid salt bridge connecting the biological specimen with the electrode, protecting tissues from leachable toxins and redox
reactions of the bare electrode. Owing to its low impedance, low
junction potential and weak polarization, silver electrodes are standard
transducers of the ionic into electric current that occurs through a
reversible redox reaction at the electrode surface.
The vibrating probe was introduced in biological studies in the 1970s. The voltage-sensitive probe is electroplated with platinum to form a
capacitive black tip ball with large surface area. When vibrating in an
artificial or natural DC voltage gradient, the capacitive ball
oscillates in a sinusoidal AC output. The amplitude of the wave is
proportional to the measuring potential difference at the frequency of
the vibration, efficiently filtered by a lock-in amplifier that boosts
probe's sensitivity.
The vibrating ion-selective microelectrode was first used in 1990 to measure calcium fluxes in various cells and tissues. The ion-selective microelectrode is an adaptation of the glass
microelectrode, where an ion-specific liquid ion exchanger (ionophore)
is tip-filled into a previously silanized (to prevent leakage)
microelectrode. Also, the microelectrode vibrates at low frequencies to
operate in the accurate self-referencing mode. Only the specific ion
permeates the ionophore,
therefore the voltage readout is proportional to the ion concentration
in the measuring condition. Then, flux is calculated using the Fick's first law.
Emerging optic-based techniques, for example, the pH optrode (or optode),
which can be integrated into a self-referencing system may become an
alternative or additional technique in bioelectricity laboratories. The
optrode does not require referencing and is insensitive to
electromagnetism simplifying system setting up and making it a suitable option for
recordings where electric stimulation is simultaneously applied.
Much work to functionally study bioelectric signaling has made
use of applied (exogenous) electric currents and fields via DC and AC
voltage-delivering apparatus integrated with agarose salt bridges. These devices can generate countless combinations of voltage magnitude
and direction, pulses, and frequencies. Currently, lab-on-a-chip
mediated application of electric fields is gaining ground in the field
with the possibility to allow high-throughput screening assays of the
large combinatory outputs.
Tools
for manipulating non-neural bioelectricity include pharmacological and
genetic reagents to alter cell connectivity (control gap junctions),
cell Vmem (control ion channels/pumps), and bioelectrically guided 2nd messengers (control neurotransmitters and other small molecules).
Fluorescence
Progress
in molecular biology over the last six decades has produced powerful
tools that facilitate the dissection of biochemical and genetic signals;
yet, they tend to not be well-suited for bioelectric studies in vivo.
Prior work relied extensively on current applied directly by
electrodes, reinvigorated by significant recent advances in materials
science and extracellular current measurements, facilitated by sophisticated self-referencing electrode systems.While electrode applications for manipulating neuraly-controlled body processes have recently attracted much attention, there are other opportunities for controlling somatic processes, as
most cell types are electrically active and respond to ionic signals
from themselves and their neighbors.
In the early part of the 21st century, a number of new molecular
techniques were developed that allowed bioelectric pathways to be
investigated with a high degree of mechanistic resolution, and to be
linked to canonical molecular cascades. These include:
Pharmacological screens to identify endogenous channels and pumps responsible for specific patterning events;
Voltage-sensitive fluorescent reporter dyes and genetically encoded
fluorescent voltage indicators for the characterization of the
bioelectric state in vivo.
Panels of well-characterized dominant ion channels that can be
misexpressed in cells of interest to alter the bioelectric state in
desired ways.
Computational platforms that are coming on-line to assist in building predictive models of bioelectric dynamics in tissues.
Compared with the electrode-based techniques, the molecular probes
provide a wider spatial resolution and facilitated dynamic analysis over
time. Although calibration or titration can be possible, molecular
probes are typically semi-quantitative, whereas electrodes provide
absolute bioelectric values. Another advantage of fluorescence
and other probes is their less-invasive nature and spatial
multiplexing, enabling the simultaneous monitoring of large areas of
embryonic or other tissues in vivo during normal or pathological pattering processes.
Roles in organisms
Early development
Work in model systems such as Xenopus laevis and zebrafish has revealed a role for bioelectric signaling in the development of heart, face, eye, brain, and other organs. Screens have identified roles for ion channels in size control of structures such as the zebrafish fin, while focused gain-of-function studies have shown for example that body
parts can be re-specified at the organ level – for example creating
entire eyes in gut endoderm. As in the brain, developmental bioelectrics can integrate information
across significant distance in the embryo, for example such as the
control of brain size by bioelectric states of ventral tissue. and the control of tumorigenesis at the site of oncogene expression by bioelectric state of remote cells.
Human disorders, as well as numerous mouse mutants show that
bioelectric signaling is important for human development (tables 1 and
2). Those effects are pervasively linked to channelopathies, which are
human disorders that result from mutations that disrupt ion channels.
Several channelopathies
result in morphological abnormalities or congenital birth defects in
addition to symptoms that affect muscle and or neurons. For example,
mutations that disrupt an inwardly rectifying potassium channelKir2.1 cause dominantly inherited Andersen–Tawil syndrome (ATS). ATS patients experience periodic paralysis, cardiac arrhythmias, and multiple morphological abnormalities that can include cleft or high arched palate, cleft or thin upper lip, flattened philtrum, micrognathia, dental oligodontia, enamel hypoplasia, delayed dentition eruption, malocclusion, broad forehead, wide set eyes, low set ears, syndactyly, clinodactyly, brachydactyly, and dysplastic kidneys. Mutations that disrupt another inwardly rectifying K+ channel Girk2 encoded by KCNJ6 cause Keppen-Lubinsky syndrome which includes microcephaly, a narrow nasal bridge, a high arched palate, and severe generalized lipodystrophy (failure to generate adipose tissue). KCNJ6 is in the Down syndrome
critical region such that duplications that include this region lead to
craniofacial and limb abnormalities and duplications that do not
include this region do not lead to morphological symptoms of Down
syndrome. Mutations in KCNH1, a voltage gated potassium channel lead to Temple-Baraitser (also known as Zimmermann- Laband) syndrome. Common features of Temple-Baraitser syndrome include absent or hypoplastic of finger and toe nails and phalanges and joint instability. Craniofacial defects associated with mutations in KCNH1 include cleft or high arched palate, hypertelorism, dysmorphic ears, dysmorphic nose, gingival hypertrophy, and abnormal number of teeth.
Mutations in CaV1.2, a voltage gated Ca2+ channel, lead to Timothy syndrome, which causes severe cardiac arrhythmia (long-QT) along with syndactyly and similar craniofacial defects to Andersen-Tawil syndrome including cleft or high-arched palate, micrognathia, low set ears, syndactyly and brachydactyly. While these channelopathies are rare, they show that functional ion
channels are important for development. Furthermore, in utero exposure
to anti-epileptic medications that target some ion channels also cause
increased incidence of birth defects such as oral clef. The effects of both genetic and exogenous disruption of ion channels
lend insight into the importance of bioelectric signaling in
development.
Wound healing and cell guidance
One
of the best-understood roles for bioelectric gradients is at the
tissue-level endogenous electric fields utilized during wound healing.
It is challenging to study wound-associated electric fields, because
these fields are weak, less fluctuating, and do not have immediate
biological responses when compared to nerve pulses and muscle
contraction. The development of the vibrating and glass microelectrodes,
demonstrated that wounds indeed produced and, importantly, sustained
measurable electric currents and electric fields. These techniques allow further characterization of the wound electric
fields/currents at cornea and skin wounds, which show active spatial and
temporal features, suggesting active regulation of these electrical
phenomena. For example, the wound electric currents are always the
strongest at the wound edge, which gradually increased to reach a peak
about 1 hour after injury. At wounds in diabetic animals, the wound electric fields are significantly compromised. Understanding the mechanisms of generation and regulation of the wound
electric currents/fields is expected to reveal new approaches to
manipulate the electrical aspect for better wound healing.
How are the electric fields at a wound produced? Epithelia
actively pump and differentially segregate ions. In the cornea
epithelium, for example, Na+ and K+ are transported inwards from tear fluid to extracellular fluid, and Cl−
is transported out of the extracellular fluid into the tear fluid. The
epithelial cells are connected by tight junctions, forming the major
electrical resistive barrier, and thus establishing an electrical
gradient across the epithelium – the transepithelial potential (TEP).Breaking the epithelial barrier, as occurs in any wounds, creates a
hole that breaches the high electrical resistance established by the
tight junctions in the epithelial sheet, short-circuiting the epithelium
locally. The TEP therefore drops to zero at the wound. However, normal
ion transport continues in unwounded epithelial cells beyond the wound
edge (typically <1 mm away), driving positive charge flow out of the
wound and establishing a steady, laterally-oriented electric field (EF)
with the cathode at the wound. Skin also generates a TEP, and when a
skin wound is made, similar wound electric currents and fields arise,
until the epithelial barrier function recovers to terminate the
short-circuit at the wound. When wound electric fields are manipulated
with pharmacological agents that either stimulate or inhibit transport
of ions, the wound electric fields also increase or decrease,
respectively. Wound healing can be speed up or slowed down accordingly
in cornea wounds.
How do electric fields affect wound healing? To heal wounds,
cells surrounding the wound must migrate and grow directionally into the
wound to cover the defect and restore the barrier. Cells important to
heal wounds respond remarkably well to applied electric fields of the
same strength that are measured at wounds. The whole gamut of cell types
and their responses following injury are affected by physiological
electric fields. Those include migration and division of epithelial
cells, sprouting and extension of nerves, and migration of leukocytes
and endothelial cells. The most well studied cellular behavior is directional migration of epithelial cells in electric fields – electrotaxis.
The epithelial cells migrate directionally to the negative pole
(cathode), which at a wound is the field polarity of the endogenous
vectorial electric fields in the epithelium, pointing (positive to
negative) to the wound center. Epithelial cells of the cornea,
keratinocytes from the skin, and many other types of cells show
directional migration at electric field strengths as low as a few mV mm−1. Large sheets of monolayerepithelial cells, and sheets of stratified multilayered epithelial cells also migrate directionally.Such collective movement closely resembles what happens during wound
healing in vivo, where cell sheets move collectively into the wound bed
to cover the wound and restore the barrier function of the skin or
cornea.
How cells sense such minute extracellular electric fields remains
largely elusive. Recent research has started to identify some genetic,
signaling and structural elements underlying how cells sense and respond
to small physiological electric fields. These include ion channels,
intracellular signaling pathways, membrane lipid rafts, and
electrophoresis of cellular membrane components.Limb regeneration in animals
In the early 20th century, Albert Mathews seminally correlated regeneration of a cnidarian polyp with the potential difference between polyp and stolon
surfaces, and affected regeneration by imposing countercurrents. Amedeo
Herlitzka, following on the wound electric currents footsteps of his
mentor, du Bois-Raymond, theorized about electric currents playing an
early role in regeneration, maybe initiating cell proliferation. Using electric fields overriding endogenous ones, Marsh and Beams
astoundingly generated double-headed planarians and even reversed the
primary body polarity entirely, with tails growing where a head
previously existed. After these seed studies, variations of the idea that bioelectricity
could sense injury and trigger or at least be a major player in
regeneration have spurred over the decades until the present day. A
potential explanation lies on resting potentials (primarily Vmem and
TEP), which can be, at least in part, dormant sensors (alarms) ready to
detect and effectors (triggers) ready to react to local damage.
Following up on the relative success of electric stimulation on
non-permissive frog leg regeneration using an implanted bimetallic rod
in the late 1960s, the bioelectric extracellular aspect of amphibian limb regeneration was
extensively dissected in the next decades. Definitive descriptive and
functional physiological data was made possible owing to the development
of the ultra-sensitive vibrating probe and improved application
devices. Amputation
invariably leads to a skin-driven outward current and a consequent
lateral electric field setting the cathode at the wound site. Although
initially pure ion leakage, an active component eventually takes place
and blocking ion translocators typically impairs regeneration. Using
biomimetic exogenous electric currents and fields, partial regeneration
was achieved, which typically included tissue growth and increased
neuronal tissue. Conversely, precluding or reverting endogenous electric
current and fields impairs regeneration.These studies in amphibian limb regeneration and related studies in lampreys and mammals combined with those of bone fracture healing and in vitro studies, led to the general rule that migrating (such as keratinocytes,
leucocytes and endothelial cells) and outgrowing (such as axons) cells
contributing to regeneration undergo electrotaxis
towards the cathode (injury original site). Congruently, an anode is
associated with tissue resorption or degeneration, as occurs in impaired
regeneration and osteoclastic resorption in bone.Despite these efforts, the promise for a significant epimorphic
regeneration in mammals remains a major frontier for future efforts,
which includes the use of wearable bioreactors to provide an environment
within which pro-regenerative bioelectric states can be driven and continued efforts at electrical stimulation.
Recent molecular work has identified proton and sodium flux as being important for tail regeneration in Xenopus tadpoles, and shown that regeneration of the entire tail (with spinal cord,
muscle, etc.) could be triggered in a range of normally non-regenerative
conditions by either molecular-genetic, pharmacological, or optogenetic methods. In planaria, work on bioelectric mechanism has revealed control of stem cell behavior, size control during remodeling, anterior-posterior polarity, and head shape. Gap junction-mediated alteration of physiological signaling produces
two-headed worms in Dugesia japonica; remarkably, these animals continue
to regenerate as two-headed in future rounds of regeneration months
after the gap junction-blocking reagent has left the tissue. This stable, long-term alteration of the anatomical layout to which
animals regenerate, without genomic editing, is an example of epigenetic
inheritance of body pattern, and is also the only available "strain" of
planarian species exhibiting an inherited anatomical change that is
different from the wild-type.
Voltage
changes can be transduced to downstream effector mechanisms via a
variety of 2nd messenger processes, including Vmem-dependent movement of
small signaling molecules like serotonin through transporters or gap
junctions, voltage-sensitive phosphatases, voltage-gated calcium
channels (which trigger calcium-signaling cascades), and dimerization of
receptors in the cell surface.Bioelectricity and genetic expression work together in an integrated fashion; nothing is downstream.Misexpression
of specific ion channels in diverse areas of frog embryos can induce
the creation of ectopic organs, such as eyes on gut tissue.
Cancer
Defection
of cells from the normally tight coordination of activity towards an
anatomical structure results in cancer; it is thus no surprise that
bioelectricity – a key mechanism for coordinating cell growth and
patterning – is a target often implicated in cancer and metastasis. Indeed, it has long been known that gap junctions have a key role in carcinogenesis and progression. Channels can behave as oncogenes and are thus suitable as novel drug targets. Recent work in amphibian models has shown that depolarization of
resting potential can trigger metastatic behavior in normal cells,while hyperpolarization (induced by ion channel misexpression, drugs,
or light) can suppress tumorigenesis induced by expression of human
oncogenes. Depolarization of resting potential appears to be a bioelectric
signature by which incipient tumor sites can be detected non-invasively. Refinement of the bioelectric signature of cancer in biomedical
contexts, as a diagnostic modality, is one of the possible applications
of this field. Excitingly, the ambivalence of polarity – depolarization as marker and
hyperpolarization as treatment – make it conceptually possible to derive
theragnostic (portmanteau of therapeutics with diagnostics) approaches,
designed to simultaneously detect and treat early tumors, in this case
based on the normalization of the membrane polarization.
Pattern regulation
Recent
experiments using ion channel opener/blocker drugs, as well as dominant
ion channel misexpression, in a range of model species, has shown that
bioelectricity, specifically, voltage gradients instruct not only stem
cell behaviorbut also large-scale patterning. Patterning cues are often mediated by spatial gradients of cell resting
potentials, or Vmem, which can be transduced into second messenger
cascades and transcriptional changes by a handful of known mechanisms.
These potentials are set by the function of ion channels and pumps, and
shaped by gap junctional connections which establish developmental
compartments (isopotential cell fields). Because both gap junctions and ion channels are themselves
voltage-sensitive, cell groups implement electric circuits with rich
feedback capabilities. The outputs of developmental bioelectric dynamics
in vivo represent large-scale patterning decisions such as the number of heads in planarian, the shape of the face in frog development, and the size of tails in zebrafish. Experimental modulation of endogenous bioelectric prepatterns have
enabled converting body regions (such as the gut) to a complete eye, inducing regeneration of appendages such as tadpole tails at non-regenerative contexts, and conversion of flatworm head shapes and contents to patterns appropriate to other species of flatworms, despite a normal genome. Recent work has shown the use of physiological modeling environments
for identifying predictive interventions to target bioelectric states
for repair of embryonic brain defects under a range of genetic and
pharmacologically induced teratologies.
Future research
Life
is ultimately an electrochemical enterprise; research in this field is
progressing along several frontiers. First is the reductive program of
understanding how bioelectric signals are produced, how voltage changes
in the cell membrane are able to regulate cell behavior, and what the
genetic and epigenetic downstream targets of bioelectric signals are. A
few mechanisms that transduce bioelectric change into alterations of
gene expression are already known, including the bioelectric control of
movement of small second-messenger molecules through cells, including
serotonin and butyrate, voltage sensitive phosphatases, among others. Also known are numerous gene targets of voltage signaling, such as Notch, BMP, FGF, and HIF-1α. Thus, the proximal mechanisms of bioelectric signaling within single cells are becoming well-understood, and advances in optogenetics and magnetogenetics continue to facilitate this research program. More challenging however
is the integrative program of understanding how specific patterns of
bioelectric dynamics help control the algorithms that accomplish
large-scale pattern regulation (regeneration and development of complex
anatomy). The incorporation of bioelectrics with chemical signaling in
the emerging field of probing cell sensory perception and
decision-making is an important frontier for future work.
Bioelectric modulation has shown control over complex
morphogenesis and remodeling, not merely setting individual cell
identity. Moreover, a number of the key results in this field have shown
that bioelectric circuits are non-local – regions of the body make
decisions based on bioelectric events at a considerable distance. Such non-cell-autonomous events suggest distributed network models of bioelectric control; new computational and conceptual paradigms may need to be developed to
understand spatial information processing in bioelectrically active
tissues. It has been suggested that results from the fields of primitive
cognition and unconventional computation are relevantto the program of cracking the bioelectric code. Finally, efforts in
biomedicine and bioengineering are developing applications such as
wearable bioreactors for delivering voltage-modifying reagents to wound
sites, and ion channel-modifying drugs (a kind of electroceutical) for repair of birth defects and regenerative repair. Synthetic biologists are likewise starting to incorporate bioelectric circuits into hybrid constructs.
The process controls the organized spatial distribution of cells during the embryonic development of an organism. Morphogenesis can take place also in a mature organism, such as in the normal maintenance of tissue by stem cells or in regeneration of tissues after damage. Cancer is an example of highly abnormal and pathological tissue morphogenesis. Morphogenesis also describes the development of unicellular life forms that do not have an embryonic stage in their life cycle. Morphogenesis is essential for the evolution of new forms.
Morphogenesis is a mechanical process involving forces that generate mechanical stress, strain, and movement of cells, and can be induced by genetic programs according to the spatial
patterning of cells within tissues. Abnormal morphogenesis is called dysmorphogenesis.
Some of the earliest ideas and mathematical descriptions on how
physical processes and constraints affect biological growth, and hence natural patterns such as the spirals of phyllotaxis, were written by D'Arcy Wentworth Thompson in his 1917 book On Growth and Form and Alan Turing in his The Chemical Basis of Morphogenesis (1952). Where Thompson explained animal body shapes as being created by varying
rates of growth in different directions, for instance to create the spiral shell of a snail,
Turing correctly predicted a mechanism of morphogenesis, the diffusion
of two different chemical signals, one activating and one deactivating
growth, to set up patterns of development, decades before the formation
of such patterns was observed. The fuller understanding of the mechanisms involved in actual organisms required the discovery of the structure of DNA in 1953, and the development of molecular biology and biochemistry.
Genetic and molecular basis
Morphogenesis is controlled by a "toolkit" of genes which switch development on and off at precise times and places. Here, gap genes in the fruit fly are switched on by genes such as bicoid, setting up stripes which create the body's segmental form.
Several types of molecules are important in morphogenesis. Morphogens
are soluble molecules that can diffuse and carry signals that control
cell differentiation via concentration gradients. Morphogens typically
act through binding to specific protein receptors. An important class of molecules involved in morphogenesis are transcription factor proteins that determine the fate of cells by interacting with DNA. These can be coded for by master regulatory genes, and either activate or deactivate the transcription
of other genes; in turn, these secondary gene products can regulate the
expression of still other genes in a regulatory cascade of gene regulatory networks. At the end of this cascade are classes of molecules that control cellular behaviors such as cell migration, or, more generally, their properties, such as cell adhesion or cell contractility. For example, during gastrulation, clumps of stem cells
switch off their cell-to-cell adhesion, become migratory, and take up
new positions within an embryo where they again activate specific cell
adhesion proteins and form new tissues and organs. Developmental
signaling pathways implicated in morphogenesis include Wnt, Hedgehog, and ephrins.
Cellular basis
Cell sorting out with cultured P19 embryonal carcinoma cells. Live cells were stained with DiI (red) or DiO (green). The red cells were genetically altered and express higher levels of E-cadherin than the green cells. The mixed culture forms large multi-cellular aggregates.
At a tissue level, ignoring the means of control, morphogenesis arises because of cellular proliferation and motility. Morphogenesis also involves changes in the cellular structure or how cells interact in tissues. These changes can result in tissue
elongation, thinning, folding, invasion or separation of one tissue into
distinct layers. The latter case is often referred as cell sorting.
Cell "sorting out" consists of cells moving so as to sort into clusters
that maximize contact between cells of the same type. The ability of
cells to do this has been proposed to arise from differential cell
adhesion by Malcolm Steinberg through his differential adhesion hypothesis. Tissue separation can also occur via more dramatic cellular differentiation events during which epithelial cells become mesenchymal (see Epithelial–mesenchymal transition).
Mesenchymal cells typically leave the epithelial tissue as a
consequence of changes in cell adhesive and contractile properties.
Following epithelial-mesenchymal transition, cells can migrate away from
an epithelium and then associate with other similar cells in a new
location. In plants, cellular morphogenesis is tightly linked to the chemical composition and the mechanical properties of the cell wall.
Cell-to-cell adhesion
During
embryonic development, cells are restricted to different layers due to
differential affinities. One of the ways this can occur is when cells
share the same cell-to-cell adhesion molecules.
For instance, homotypic cell adhesion can maintain boundaries between
groups of cells that have different adhesion molecules. Furthermore,
cells can sort based upon differences in adhesion between the cells, so
even two populations of cells with different levels of the same adhesion
molecule can sort out. In cell culture
cells that have the strongest adhesion move to the center of a mixed
aggregates of cells. Moreover, cell-cell adhesion is often modulated by
cell contractility, which can exert forces on the cell-cell contacts so
that two cell populations with equal levels of the same adhesion
molecule can sort out. The molecules responsible for adhesion are called
cell adhesion molecules (CAMs). Several types of cell adhesion
molecules are known and one major class of these molecules are cadherins.
There are dozens of different cadherins that are expressed on different
cell types. Cadherins bind to other cadherins in a like-to-like manner:
E-cadherin
(found on many epithelial cells) binds preferentially to other
E-cadherin molecules. Mesenchymal cells usually express other cadherin
types such as N-cadherin.
Extracellular matrix
The extracellular matrix (ECM) is involved in keeping tissues separated, providing structural support or providing a structure for cells to migrate on. Collagen, laminin, and fibronectin
are major ECM molecules that are secreted and assembled into sheets,
fibers, and gels. Multisubunit transmembrane receptors called integrins
are used to bind to the ECM. Integrins bind extracellularly to
fibronectin, laminin, or other ECM components, and intracellularly to microfilament-binding proteins α-actinin and talin to link the cytoskeleton with the outside. Integrins also serve as receptors to trigger signal transduction cascades when binding to the ECM. A well-studied example of morphogenesis that involves ECM is mammary gland ductal branching.
Cell contractility
Tissues can change their shape and separate into distinct layers via cell contractility. Just as in muscle cells, myosin
can contract different parts of the cytoplasm to change its shape or
structure. Myosin-driven contractility in embryonic tissue morphogenesis
is seen during the separation of germ layers in the model organismsCaenorhabditis elegans, Drosophila and zebrafish.
There are often periodic pulses of contraction in embryonic
morphogenesis. A model called the cell state splitter involves
alternating cell contraction and expansion, initiated by a bistable
organelle at the apical end of each cell. The organelle consists of microtubules and microfilaments
in mechanical opposition. It responds to local mechanical perturbations
caused by morphogenetic movements. These then trigger traveling embryonic differentiation waves
of contraction or expansion over presumptive tissues that determine
cell type and is followed by cell differentiation. The cell state
splitter was first proposed to explain neural plate morphogenesis during gastrulation of the axolotl and the model was later generalized to all of morphogenesis.
In the development of the lung a bronchus branches into bronchioles forming the respiratory tree. The branching is a result of the tip of each bronchiolar tube
bifurcating, and the process of branching morphogenesis forms the
bronchi, bronchioles, and ultimately the alveoli.
Branching morphogenesis is also evident in the ductal formation of the mammary gland.Primitive duct formation begins in development, but the branching formation of the duct system begins later in response to estrogen during puberty and is further refined in line with mammary gland development.
Cancer morphogenesis
Cancer can result from disruption of normal morphogenesis, including both tumor formation and tumor metastasis. Mitochondrial dysfunction can result in increased cancer risk due to disturbed morphogen signaling.
Virus morphogenesis
During assembly of the bacteriophage (phage) T4virion, the morphogenetic proteins encoded by the phage genes
interact with each other in a characteristic sequence. Maintaining an
appropriate balance in the amounts of each of these proteins produced
during viral infection appears to be critical for normal phage T4
morphogenesis. Phage T4 encoded proteins that determine virion structure include
major structural components, minor structural components and
non-structural proteins that catalyze specific steps in the
morphogenesis sequence. Phage T4 morphogenesis is divided into three independent pathways: the
head, the tail and the long tail fibres as detailed by Yap and Rossman.
Another famous model is the so-called French flag model, developed in the sixties.
Improvements in computer performance
in the twenty-first century enabled the simulation of relatively
complex morphogenesis models. In 2020, such a model was proposed where
cell growth and differentiation is that of a cellular automaton with parametrized rules. As the rules' parameters are differentiable, they can be trained with gradient descent, a technique which has been highly optimized in recent years due to its use in machine learning. This model was limited to the generation of pictures, and is thus bi-dimensional.
A similar model to the one described above was subsequently
extended to generate three-dimensional structures, and was demonstrated
in the video game Minecraft, whose block-based nature made it particularly expedient for the simulation of 3D cellular automatons.
