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Suicide gene

From Wikipedia, the free encyclopedia

In the field of genetics, a suicide gene is a gene that will cause a cell to kill itself through the process of apoptosis (programmed cell death). Activation of a suicide gene can cause death through a variety of pathways, but one important cellular "switch" to induce apoptosis is the p53 protein. Stimulation or introduction (through gene therapy) of suicide genes is a potential way of treating cancer or other proliferative diseases.

Suicide genes form the basis of a strategy for making cancer cells more vulnerable or sensitive to chemotherapy. The approach has been to attach parts of genes expressed in cancer cells to other genes for enzymes not found in mammals that can convert a harmless substance into one that is toxic to the tumor.[1] Most suicide genes mediate this sensitivity by coding for viral or bacterial enzymes that convert an inactive drug into toxic antimetabolites that inhibit the synthesis of nucleic acid. Suicide genes must be introduced into the cells in ways that ensure their uptake and expression by as many cancer cells as possible, while limiting their expression by normal cells. Suicide gene therapy for cancer requires the vector to have the capacity to discriminate between target and non target cells, between the cancer cells and normal cells.[2]

Apoptosis

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Cell death can majorly occur by either necrosis or apoptosis. Necrosis occurs when a cell is damaged by an external force, such as poison, a bodily injury, an infection or getting cut off from blood supply. When cells die from necrosis, it's a rather messy affair. The death causes inflammation that can cause further distress of injury within the body. Whereas, apoptosis causes degradation of cellular components without eliciting an inflammatory response.[3]

Many cells undergo programmed cell death, or apoptosis, during fetal development. A form of cell death in which a programmed sequence of events leads to the elimination of cells without releasing harmful substances into the surrounding. Apoptosis plays a crucial role in developing and maintaining the health of the body by eliminating old cells, unnecessary cells, and unhealthy cells. The human body replaces perhaps one million cells per second. When a cell is compelled to commit suicide, proteins called caspases go into action. They break down the cellular components needed for survival, and they spur production of enzymes known as DNase, which destroy the DNA in the nucleus of the cell. The cell shrinks and sends out distress signals, which are answered by macrophages. The macrophages clean away the shrunken cells, leaving no trace, so these cells do not damage surrounding necrotic cells do. Apoptosis is also essential to prenatal development. For example, in embryos, fingers and toes are initially connected to adjacent digits by tissue. The cells of this connecting tissue undergo apoptosis to produce separate digits. In brain development, initially millions of extra neurons are created. The cells that don't form synaptic connections undergo apoptosis. Programmed cell death is also necessary to start the process of menstruation. That's not to say that apoptosis is a perfect process. Rather than dying due to injury, cells that go through apoptosis die in response to signals within the body. When cells recognize viruses and gene mutations, they may induce death to prevent the damage from spreading. Scientist are trying to learn how they can modulate apoptosis, so that they can control which cells live and which undergo programmed cell death. Anti-cancer drugs and radiation, for example, work by triggering apoptosis in diseased cells. Many diseases and disorders are linked with the life and death of cells—increased apoptosis is a characteristic of AIDS, Alzheimer's, and Parkinson's disease, while decreased apoptosis can signal lupus or cancer. Understanding how to regulate apoptosis could be the first step to treating these conditions.[4]

Too little or too much apoptosis can play a role in many diseases. When apoptosis does not work correctly, cells that should be eliminated may persist and become immortal, for example, in cancer and leukemia. when apoptosis works overly well, it kills too many cells and inflicts grave tissue damage. This is the case in strokes and neurodegenerative disorders such as Alzheimer's, Huntington's, and Parkinson's disease. Also known as programmed cell death and cell suicide.[5]

Applications

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Cancer suicide gene therapy

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The ultimate goal of cancer therapy is the complete elimination of all cancer cells, while leaving all healthy cells unharmed. One of the most promising therapeutic strategies in this regard is cancer suicide gene therapy (CSGT), which is rapidly progressing into new frontiers. The therapeutic success, in CSGT, is primarily contingent upon precision in delivery of the therapeutic transgenes to the cancer cells only. This is addressed by discovering and targeting unique or / and over-expressed biomarkers displayed on the cancer cells and cancer stem cells. Specificity of cancer therapeutic effects is further enhanced by designing the DNA constructs, which put the therapeutic genes under the control of the cancer cell specific promoters. The delivery of the suicidal genes to the cancer cells involves viral, as well as synthetic vectors, which are guided by cancer specific antibodies and ligands. The delivery options also include engineered stem cells with tropisms towards cancers. Main mechanisms inducing cancer cells' deaths include: transgenic expression of thymidine kinases, cytosine deaminases, intracellular antibodies, telomeraseses, caspases, DNases. Precautions are undertaken to eliminate the risks associated with transgenesis. Progress in genomics and proteomics should help us in identifying the cancer specific biomarkers and metabolic pathways for developing new strategies towards clinical trials of targeted and personalized gene therapy of cancer. By introducing the gene into a malignant tumor, the tumor would reduce in size and possibly disappear completely, provided all the individual cells have received a copy of the gene.

When the DNA sample in the virus is taken from the patient's own healthy cells, the virus does not need to be able to differentiate between cancer cells and healthy ones. In addition, the advantage is that it is also able to prevent metastasis upon the death of a tumor.

As a cancer treatment

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Indirect gene therapy

One of the challenges of cancer treatment is how to destroy malignant tumors without damaging healthy cells. A new method that shows great promise for accomplishing this employs the use of a suicide gene. A suicide gene is a gene which will cause a cell to kill itself through apoptosis. Suicide gene therapy involves delivery of a gene which codes for a cytotoxic product into tumor cells.[6] This can be achieved by two approaches, indirect gene therapy and direct gene therapy. Indirect gene therapy employs enzyme-activated prodrug, in which the enzyme converts the prodrug to a toxic substance and the gene coding for this enzyme is delivered to the tumor cells. For example, a commonly studied strategy based on transfection of herpes simplex virus thymidine kinase (HSV-TK) along with administration of ganciclovir (GSV), in which HSK-TK assists in converting GCV to a toxic compound that inhibits DNA synthesis and causes cell death.[7][6][8] Whereas, direct gene therapy employs a toxin gene or a gene which has the ability to correct mutated proapoptotic genes, which can in turn induce cell death via apoptosis.  For instance, the most researched immunotoxin for cancer therapy is the diphtheria toxin as it inhibits protein synthesis by inactivating elongation factor 2 (EF-2) which in turn inhibits protein translation,[6][9] Moreover, p53 is identified to be frequently abnormal in human tumors and studies show that restoring function of p53 can cause apoptosis of cancer cells.[6] Suicide gene therapy is not necessarily expected to eliminate the need for chemotherapy and radiation treatment for all cancerous tumors. The damage inflicted upon the tumor cells, however, makes them more susceptible to the chemo or radiation. This approach has already proven effective against prostate and bladder cancers. The application of suicide gene therapy is being expanded to several other forms of cancer as well. Cancer patients often experience depressed immune systems, so they can suffer some side effects of the use of a virus as a delivery agent.[citation needed]

Direct gene therapy
Bystander effect

Improved vectors

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Suicide gene delivery can be broadly classified into three groups which include viral vectors, synthetic vectors and cell-based vectors.[6] The most efficient vehicles for gene delivery are viral vectors. Widely used viruses for gene therapy include retrovirus, adenovirus (Ads), lentivirus and Aden-associated viruses (AAVs). Non-viral vectors like synthetic vectors were used to combat certain disadvantages of viral vectors like immunogenicity, insertional mutagenesis to name a few. Synthetic vectors refer to use of nanoparticles, like gold nanoparticles, to delivery genes to target cells.[10] Lastly, cell-based vectors employ stem cells as carriers of suicide genes. In the last few years, cell-mediated gene therapy for cancer using mesenchymal stem cells (MSCs) was patented.[11]

Bystander effect

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The bystander effect (BE) is phenomenon as a result of which it is possible to kill untransfected tumor cells located adjacent to transduced cells in suicide gene therapy.[8][12][13] As hundred percent transduction of all tumor cells is very difficult to achieve, BE is critical feature of suicide gene therapy.

Limitations

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The drug is supposed to show high specificity towards cancer in order to effective, but studies have shown this to be rarely achieved. Moreover, expression of suicide gene was under control of tumor-specific promoters like human telomerase (hTERT), osteocalcin, carcinoembryonic antigen; however, only hTERT promoter was found to enter clinic trials.[14] This is majorly because of the low transcriptional power of these tumor-specific promoters for suicide gene expression. Additionally, poor accessibility to target cells is an important limitation of suicide gene therapy. Another major hurdle of suicide gene therapy is partial vector specificity to target affected cells. Finally, lack of specific animal models to predict the clinical outcome and other effects of SGT.

Biotechnology

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Suicide genes are often utilized in biotechnology to assist in molecular cloning. Vectors incorporate suicide genes for an organism (such as E. coli). The cloning project focuses on replacing the suicide gene by the desired fragment. Selection of vectors carrying the desired fragment is improved since vectors retaining the suicide gene result in cell death.

References

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  1. ^ Karjoo Z, Chen X, Hatefi A (April 2016). "Progress and problems with the use of suicide genes for targeted cancer therapy". Advanced Drug Delivery Reviews. 99 (Pt A): 113–128. doi:10.1016/j.addr.2015.05.009. PMC 4758904. PMID 26004498.
  2. ^ "Suicide gene". MedicineNet. Retrieved 15 November 2014.
  3. ^ Fink SL, Cookson BT (April 2005). "Apoptosis, pyroptosis, and necrosis: mechanistic description of dead and dying eukaryotic cells". Infection and Immunity. 73 (4): 1907–1916. doi:10.1128/IAI.73.4.1907-1916.2005. PMC 1087413. PMID 15784530.
  4. ^ "What is apoptosis?". HowStuffWorks. 2010-03-31. Retrieved 15 November 2014.
  5. ^ "Apoptosis definition". Medical Dictionary: Definitions of Popular Terms Defined on MedTerms. Medicinenet.com. Retrieved 15 November 2014.
  6. ^ a b c d e Navarro SA, Carrillo E, Griñán-Lisón C, Martín A, Perán M, Marchal JA, Boulaiz H (September 2016). "Cancer suicide gene therapy: a patent review". Expert Opinion on Therapeutic Patents. 26 (9): 1095–1104. doi:10.1080/13543776.2016.1211640. PMID 27424657. S2CID 1495377.
  7. ^ Düzgüneş N (2019). "Origins of Suicide Gene Therapy". In Düzgüneş N (ed.). Suicide Gene Therapy: Methods and Protocols. Methods in Molecular Biology. Vol. 1895. New York, NY: Springer. pp. 1–9. doi:10.1007/978-1-4939-8922-5_1. ISBN 978-1-4939-8922-5. PMID 30539525. S2CID 54473687.
  8. ^ a b Vassaux G, Martin-Duque P (April 2004). "Use of suicide genes for cancer gene therapy: study of the different approaches". Expert Opinion on Biological Therapy. 4 (4): 519–530. doi:10.1517/14712598.4.4.519. PMID 15102601. S2CID 29442217.
  9. ^ Lin B, Gao A, Zhang R, Ma H, Shen H, Hu Q, et al. (August 2015). "Use of a Novel Integrase-Deficient Lentivirus for Targeted Anti-Cancer Therapy With Survivin Promoter-Driven Diphtheria Toxin A". Medicine. 94 (31): e1301. doi:10.1097/MD.0000000000001301. PMC 4616595. PMID 26252309.
  10. ^ Vago R, Collico V, Zuppone S, Prosperi D, Colombo M (September 2016). "Nanoparticle-mediated delivery of suicide genes in cancer therapy". Pharmacological Research. 111: 619–641. doi:10.1016/j.phrs.2016.07.007. PMID 27436147.
  11. ^ Moradian Tehrani R, Verdi J, Noureddini M, Salehi R, Salarinia R, Mosalaei M, et al. (May 2018). "Mesenchymal stem cells: A new platform for targeting suicide genes in cancer". Journal of Cellular Physiology. 233 (5): 3831–3845. doi:10.1002/jcp.26094. PMID 28703313. S2CID 46865654.
  12. ^ Hossain JA, Marchini A, Fehse B, Bjerkvig R, Miletic H (January 2020). "Suicide gene therapy for the treatment of high-grade glioma: past lessons, present trends, and future prospects". Neuro-Oncology Advances. 2 (1): vdaa013. doi:10.1093/noajnl/vdaa013. PMC 7212909. PMID 32642680.
  13. ^ Singhal, Sunil; Kaiser, Larry R. (1998-07-01). "Cancer Chemotherapy Using Suicide Genes". Surgical Oncology Clinics of North America. Cancer Gene Therapy. 7 (3): 505–536. doi:10.1016/S1055-3207(18)30258-8. ISSN 1055-3207. PMID 9624215.
  14. ^ Saeb, Sepideh; Assche, Jeanne Van; Loustau, Thomas; Rohr, Olivier; Wallet, Clémentine; Schwartz, Christian (2022-03-01). "Suicide gene therapy in cancer and HIV-1 infection: An alternative to conventional treatments". Biochemical Pharmacology. 197: 114893. doi:10.1016/j.bcp.2021.114893. ISSN 0006-2952. PMID 34968484. S2CID 245548079.