RNA-directed DNA polymerase | |
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A conceptual diagram showing the protein component of telomerase (TERT) in grey and the RNA component (TR) in yellow
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Identifiers | |
EC number | 2.7.7.49 |
CAS number | 9068-38-6 |
Databases | |
IntEnz | IntEnz view |
BRENDA | BRENDA entry |
ExPASy | NiceZyme view |
KEGG | KEGG entry |
MetaCyc | metabolic pathway |
PRIAM | profile |
PDB structures | RCSB PDB PDBe PDBsum |
Gene Ontology | AmiGO / QuickGO |
Telomerase, also called terminal transferase, is a ribonucleoprotein that adds a species-dependent telomere repeat sequence to the 3' end of telomeres. A telomere is a region of repetitive sequences at each end of eukaryotic chromosomes in most eukaryotes. Telomeres protect the end of the chromosome from DNA damage or from fusion with neighbouring chromosomes. The fruit fly Drosophila melanogaster lacks telomerase, but instead uses retrotransposons to maintain telomeres.
Telomerase is a reverse transcriptase enzyme that carries its own RNA molecule (e.g., with the sequence 3′-CCCAAUCCC-5′ in Trypanosoma brucei) which is used as a template when it elongates telomeres. Telomerase is active in normal stem cells and most cancer cells, but is normally absent from, or at very low levels in, most somatic cells.
History
The existence of a compensatory mechanism for telomere shortening was first found by Soviet biologist Alexey Olovnikov in 1973, who also suggested the telomere hypothesis of aging and the telomere's connections to cancer.
Telomerase in the ciliate Tetrahymena was discovered by Carol W. Greider and Elizabeth Blackburn in 1984. Together with Jack W. Szostak, Greider and Blackburn were awarded the 2009 Nobel Prize in Physiology or Medicine for their discovery.
The role of telomeres and telomerase in cell aging and cancer was established by scientists at biotechnology company Geron with the cloning of the RNA and catalytic components of human telomerase and the development of a polymerase chain reaction (PCR) based assay for telomerase activity called the TRAP assay, which surveys telomerase activity in multiple types of cancer.
The negative stain electron microscopy (EM) structures of human and Tetrahymena telomerases were characterized in 2013. Two years later, the first cryo-electron microscopy (cryo-EM) structure of telomerase holoenzyme (Tetrahymena) was determined. In 2018, the structure of human telomerase was determined through cryo-EM by UC Berkeley scientists.
Human telomerase structure
The
molecular composition of the human telomerase complex was determined by
Scott Cohen and his team at the Children's Medical Research Institute
(Sydney Australia) and consists of two molecules each of human telomerase reverse transcriptase (TERT), telomerase RNA (TR or TERC), and dyskerin (DKC1). The genes of telomerase subunits, which include TERT, TERC, DKC1 and TEP1, are located on different chromosomes. The human TERT gene (hTERT) is translated into a protein of 1132 amino acids. TERT polypeptide folds with (and carries) TERC, a non-coding RNA (451 nucleotides long). TERT has a 'mitten' structure that allows it to wrap around the chromosome to add single-stranded telomere repeats.
TERT is a reverse transcriptase, which is a class of enzyme that creates single-stranded DNA using single-stranded RNA as a template.
The protein consists of four conserved domains (RNA-Binding Domain
(TRBD), fingers, palm and thumb), organized into a ring configuration
that shares common features with retroviral reverse transcriptases, viral RNA polymerases and bacteriophage B-family DNA polymerases.
TERT proteins from many eukaryotes have been sequenced.
Mechanism
By using TERC, TERT can add a six-nucleotide repeating sequence, 5'-TTAGGG
(in vertebrates, the sequence differs in other organisms) to the 3'
strand of chromosomes. These TTAGGG repeats (with their various protein
binding partners) are called telomeres. The template region of TERC is
3'-CAAUCCCAAUC-5'.
Telomerase can bind the first few nucleotides of the template to
the last telomere sequence on the chromosome, add a new telomere repeat
(5'-GGTTAG-3') sequence, let go, realign the new 3'-end of telomere to
the template, and repeat the process. Telomerase reverses telomere shortening.
Clinical implications
Aging
Telomerase replaces short bits of DNA known as telomeres, which are otherwise shortened when a cell divides via mitosis.
In normal circumstances, where telomerase is absent, if a cell divides recursively, at some point the progeny reach their Hayflick limit, which is believed to be between 50–70 cell divisions. At the limit the cells become senescent and cell division stops.
Telomerase allows each offspring to replace the lost bit of DNA,
allowing the cell line to divide without ever reaching the limit. This
same unbounded growth is a feature of cancerous growth.
Embryonic stem cells
express telomerase, which allows them to divide repeatedly and form the
individual. In adults, telomerase is highly expressed only in cells
that need to divide regularly, especially in male sperm cells but also in epidermal cells, in activated T cell and B cell lymphocytes, as well as in certain adult stem cells, but in the great majority of cases somatic cells do not express telomerase.
A comparative biology study of mammalian telomeres indicated that
telomere length of some mammalian species correlates inversely, rather
than directly, with lifespan, and concluded that the contribution of
telomere length to lifespan is unresolved. Telomere shortening does not occur with age in some postmitotic tissues, such as in the rat brain. In humans, skeletal muscle telomere lengths remain stable from ages 23 –74.
In baboon skeletal muscle, which consists of fully differentiated
post-mitotic cells, less than 3% of myonuclei contain damaged telomeres
and this percentage does not increase with age.
Thus, telomere shortening does not appear to be a major factor in the
aging of the differentiated cells of brain or skeletal muscle. In human
liver, cholangiocytes and hepatocytes show no age-related telomere shortening.
Another study found little evidence that, in humans, telomere length is
a significant biomarker of normal aging with respect to important
cognitive and physical abilities.
Some experiments have raised questions on whether telomerase can
be used as an anti-aging therapy, namely, the fact that mice with
elevated levels of telomerase have higher cancer incidence and hence do
not live longer. Telomerase also favors tumorogenesis, which leads to questions about its potential as an anti-aging therapy.
On the other hand, one study showed that activating telomerase in
cancer-resistant mice by overexpressing its catalytic subunit extended
lifespan.
A study that focused on Ashkenazi Jews found that long-lived subjects inherited a hyperactive version of telomerase.
Premature aging
Premature aging syndromes including Werner syndrome, Ataxia telangiectasia, Ataxia-telangiectasia like disorder, Bloom syndrome, Fanconi anemia and Nijmegen breakage syndrome are associated with short telomeres. However, the genes that have mutated in these diseases all have roles in the repair of DNA damage and the increased DNA damage may, itself, be a factor in the premature aging. An additional role in maintaining telomere length is an active area of investigation.
Cancer
In vitro, when cells approach the Hayflick limit, the time to senescence can be extended by inactivating the tumor suppressor proteins - p53 and Retinoblastoma protein (pRb). Cells
that have been so-altered eventually undergo an event termed a "crisis"
when the majority of the cells in the culture die. Sometimes, a cell
does not stop dividing once it reaches crisis. In a typical situation,
the telomeres are shortened
and chromosomal integrity declines with every subsequent cell division.
Exposed chromosome ends are interpreted as double-stranded breaks (DSB)
in DNA; such damage is usually repaired
by reattaching (religating) the broken ends together. When the cell
does this due to telomere-shortening, the ends of different chromosomes
can be attached to each other. This solves the problem of lacking
telomeres, but during cell division anaphase, the fused chromosomes are randomly ripped apart, causing many mutations
and chromosomal abnormalities. As this process continues, the cell's
genome becomes unstable. Eventually, either fatal damage is done to the
cell's chromosomes (killing it via apoptosis), or an additional mutation that activates telomerase occurs.
With telomerase activation some types of cells and their offspring become immortal (bypass the Hayflick limit), thus avoiding cell death as long as the conditions for their duplication are met. Many cancer cells
are considered 'immortal' because telomerase activity allows them to
live much longer than any other somatic cell, which, combined with
uncontrollable cell proliferation is why they can form tumors. A good example of immortal cancer cells is HeLa cells, which have been used in laboratories as a model cell line since 1951.
While this method of modeling human cancer in cell culture is
effective and has been used for many years by scientists, it is also
very imprecise. The exact changes that allow for the formation of the
tumorigenic clones
in the above-described experiment are not clear. Scientists addressed
this question by the serial introduction of multiple mutations present
in a variety of human cancers. This has led to the identification of
mutation combinations that form tumorigenic cells in a variety of cell
types. While the combination varies by cell type, the following
alterations are required in all cases: TERT activation, loss of p53
pathway function, loss of pRb pathway function, activation of the Ras or myc proto-oncogenes, and aberration of the PP2A protein phosphatase.
That is to say, the cell has an activated telomerase, eliminating the
process of death by chromosome instability or loss, absence of
apoptosis-induction pathways, and continued mitosis activation.
This model of cancer
in cell culture accurately describes the role of telomerase in actual
human tumors. Telomerase activation has been observed in ~90% of all
human tumors,
suggesting that the immortality conferred by telomerase plays a key
role in cancer development. Of the tumors without TERT activation, most employ a separate pathway to maintain telomere length termed Alternative Lengthening of Telomeres (ALT ).
The exact mechanism behind telomere maintenance in the ALT pathway is
unclear, but likely involves multiple recombination events at the
telomere.
Elizabeth Blackburn et al.,
identified the upregulation of 70 genes known or suspected in cancer
growth and spread through the body, and the activation of glycolysis,
which enables cancer cells to rapidly use sugar to facilitate their
programmed growth rate (roughly the growth rate of a fetus).
Approaches to controlling telomerase and telomeres for cancer therapy include gene therapy, immunotherapy, small-molecule and signal pathway inhibitors.
Drugs
The ability to maintain functional telomeres may be one mechanism that allows cancer cells to grow in vitro for decades. Telomerase activity is necessary to preserve many cancer types and is inactive in somatic cells, creating the possibility that telomerase inhibition could selectively repress cancer cell growth with minimal side effects.
If a drug can inhibit telomerase in cancer cells, the telomeres of
successive generations will progressively shorten, limiting tumor
growth.
Telomerase is a good biomarker
for cancer detection because most human cancers cells express high
levels of it. Telomerase activity can be identified by its catalytic
protein domain (hTERT). This is the rate-limiting step in telomerase activity. It is associated with many cancer types. Various cancer cells and fibroblasts transformed with hTERT cDNA
have high telomerase activity, while somatic cells do not. Cells
testing positive for hTERT have positive nuclear signals. Epithelial
stem cell tissue and its early daughter cells are the only noncancerous
cells in which hTERT can be detected. Since hTERT expression is
dependent only on the number of tumor cells within a sample, the amount
of hTERT indicates the severity of a cancer.
The expression of hTERT can also be used to distinguish benign tumors from malignant tumors. Malignant tumors have higher hTERT expression than benign tumors. Real-time reverse transcription polymerase chain reaction (RT-PCR) quantifying hTERT expression in various tumor samples verified this varying expression.
The lack of telomerase does not affect cell growth, until the
telomeres are short enough to cause cells to “die or undergo growth
arrest”. However, inhibiting telomerase alone is not enough to destroy
large tumors. It must be combined with surgery, radiation, chemotherapy, or immunotherapy.
Cells may reduce their telomere length by only 50-252 base pairs per cell division, which can lead to a long lag phase.
Immunotherapy
Immunotherapy successfully treats some kinds of cancer, such as melanoma. This treatment involves manipulating a human’s immune system to destroy cancerous cells. Humans have two major antigen identifying lymphocytes: CD8+ cytotoxic T-lymphocytes (CTL) and CD4+ helper T-lymphocytes that can destroy cells. Antigen receptors on CTL can bind to a 9-10 amino acid chain that is presented by the major histocompatibility complex
(MHC) as in Figure 4. HTERT is a potential target antigen.
Immunotargeting should result in relatively few side effects since hTERT
expression is associated only with telomerase and is not essential in
almost all somatic cells. GV1001 uses this pathway. Experimental drug and vaccine therapies targeting active telomerase have been tested in mouse models, and clinical trials have begun. One drug, imetelstat, is being clinically researched as a means of interfering with telomerase in cancer cells.
Most of the harmful cancer-related effects of telomerase are dependent
on an intact RNA template. Cancer stem cells that use an alternative
method of telomere maintenance are still killed when telomerase's RNA
template is blocked or damaged.
Telomerase Vaccines
Two telomerase vaccines have been developed: GRNVAC1 and GV1001. GRNVAC1 isolates dendritic cells and the RNA that codes for the telomerase protein and puts them back into the patient to make cytotoxic
T cells that kill the telomerase-active cells. GV1001 is a peptide from
the active site of hTERT and is recognized by the immune system that
reacts by killing the telomerase-active cells.
Targeted apoptosis
Another independent approach is to use oligoadenylated anti-telomerase antisense oligonucleotides and ribozymes to target telomerase RNA, reducing dissociation and apoptosis
(Figure 5). The fast induction of apoptosis through antisense binding
may be a good alternative to the slower telomere shortening.
Small interfering RNA (siRNA)
siRNAs
are small RNA molecules that induce the sequence-specific degradation
of other RNAs. siRNA treatment can function similar to traditional gene therapy
by destroying the mRNA products of particular genes, and therefore
preventing the expression of those genes. A 2012 study found that
targeting TERC with an siRNA reduced telomerase activity by more than
50% and resulted in decreased viability of immortal cancer cells.
Treatment with both the siRNA and radiation caused a greater reduction
in tumor size in mice than treatment with radiation alone, suggesting
that targeting telomerase could be a way to increase the efficacy of
radiation in treating radiation-resistant tumors.
Heart disease, diabetes and quality of life
Blackburn
also discovered that mothers caring for very sick children have shorter
telomeres when they report that their emotional stress is at a maximum
and that telomerase was active at the site of blockages in coronary
artery tissue, possibly accelerating heart attacks.
In 2009, it was shown that the amount of telomerase activity
significantly increased following psychological stress. Across the
sample of patients telomerase activity in increased peripheral blood
mononuclear cells by 18% one hour after the end of the stress.
A study in 2010 found that there was "significantly greater"
telomerase activity in participants than controls after a three-month
meditation retreat.
Telomerase deficiency has been linked to diabetes mellitus and impaired insulin secretion in mice, due to loss of pancreatic insulin-producing cells.
Rare human diseases
Mutations in TERT have been implicated in predisposing patients to aplastic anemia, a disorder in which the bone marrow fails to produce blood cells, in 2005.
Cri du chat syndrome
(CdCS) is a complex disorder involving the loss of the distal portion
of the short arm of chromosome 5. TERT is located in the deleted region,
and loss of one copy of TERT has been suggested as a cause or
contributing factor of this disease.
Dyskeratosis congenita (DC) is a disease of the bone marrow that can be caused by some mutations in the telomerase subunits. In the DC cases, about 35% cases are X-linked-recessive on the DKC1 locus and 5% cases are autosomal dominant on the TERT and TERC loci.
Patients with DC have severe bone marrow failure manifesting as abnormal skin pigmentation, leucoplakia (a white thickening of the oral mucosa) and nail dystrophy,
as well as a variety of other symptoms. Individuals with either TERC
or DKC1 mutations have shorter telomeres and defective telomerase
activity in vitro versus other individuals of the same age.
In one family autosomal dominant DC was linked to a heterozygous TERT mutation.
These patients also exhibited an increased rate of telomere-shortening,
and genetic anticipation (i.e., the DC phenotype worsened with each
generation).