Int J Genomics

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Int J Genomics. 2016; 2016: 2405954.

Published online 2016 Dec 8. doi: 10.1155/2016/2405954

PMCID: PMC5178364

PMID: 28053975

Role of Recombinant DNA Technology to Improve Life

Suliman Khan, 1 Muhammad Wajid Ullah, 2 Rabeea Siddique, 3 Ghulam Nabi, 1 Sehrish Manan, 4Muhammad

Yousaf, 5 and Hongwei Hou 1 , *

Author information Article notes Copyright and License information Disclaimer

This article has been cited by other articles in PMC.

Abstract
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1. Introduction
Human life is greatly affected by three factors: deficiency of food, health problems, and environmental issues. Food
and health are basic human requirements beside a clean and safe environment. With increasing world's population at
a greater rate, human requirements for food are rapidly increasing. Humans require safe-food at reasonable price.
Several human related health issues across the globe cause large number of deaths. Approximately 36 million people
die each year from noncommunicable and communicable diseases, such as cardiovascular diseases, cancer, diabetes,
AIDS/HIV, tuberculosis, malaria, and several others according to http://GlobalIssues.org/. Despite extensive efforts
being made, the current world food production is much lower than human requirements, and health facilities are
even below standard in the third-world countries. Rapid increase in industrialization has soared up the
environmental pollution and industrial wastes are directly allowed to mix with water, which has affected aquatic
marines and, indirectly, human-beings. Therefore, these issues urge to be addressed through modern technologies.
Unlike tradition approaches to overcome agriculture, health, and environmental issues through breeding, traditional
medicines, and pollutants degradation through conventional techniques respectively, the genetic engineering utilizes
modern tools and approaches, such as molecular cloning and transformation, which are less time consuming and
yield more reliable products. For example, compared to conventional breeding that transfers a large number of both
specific and nonspecific genes to the recipient, genetic engineering only transfers a small block of desired genes to
the target through various approaches, such as biolistic and Agrobacterium-mediated transformation [1]. The
alteration into plant genomes is brought either by homologous recombination dependent gene targeting or by
nuclease-mediated site-specific genome modification. Recombinase mediated site-specific genome integration and
oligonucleotide directed mutagenesis can also be used [2].
Recombinant DNA technology is playing a vital role in improving health conditions by developing new vaccines
and pharmaceuticals. The treatment strategies are also improved by developing diagnostic kits, monitoring devices,
and new therapeutic approaches. Synthesis of synthetic human insulin and erythropoietin by genetically modified
bacteria [3] and production of new types of experimental mutant mice for research purposes are one of the leading
examples of genetic engineering in health. Likewise, genetic engineering strategies have been employed to tackle
the environmental issues such as converting wastes into biofuels and bioethanol [4–7], cleaning the oil spills,
carbon, and other toxic wastes, and detecting arsenic and other contaminants in drinking water. The genetically
modified microbes are also effectively used in biomining and bioremediation.
The advent of recombinant DNA technology revolutionized the development in biology and led to a series of
dramatic changes. It offered new opportunities for innovations to produce a wide range of therapeutic products with
immediate effect in the medical genetics and biomedicine by modifying microorganisms, animals, and plants to
yield medically useful substances [8, 9]. Most biotechnology pharmaceuticals are recombinant in nature which plays
a key role against human lethal diseases. The pharmaceutical products synthesized through recombinant DNA
technology, completely changed the human life in such a way that the U.S. Food and Drug Administration (FDA)
approved more recombinant drugs in 1997 than in the previous several years combined, which includes anemia,
AIDS, cancers (Kaposi's sarcoma, leukemia, and colorectal, kidney, and ovarian cancers), hereditary disorders
(cystic fibrosis, familial hypercholesterolemia, Gaucher's disease, hemophilia A, severe combined
immunodeficiency disease, and Turnor's syndrome), diabetic foot ulcers, diphtheria, genital warts, hepatitis B,
hepatitis C, human growth hormone deficiency, and multiple sclerosis. Considering the plants develop multigene
transfer, site-specific integration and specifically regulated gene expression are crucial advanced approaches [10].
Transcriptional regulation of endogenous genes, their effectiveness in the new locations, and the precise control of
transgene expression are major challenges in plant biotechnology which need further developments for them to be
used successfully [11].
Human life is greatly threatened by various factors, like food limitations leading to malnutrition, different kinds of
lethal diseases, environmental problems caused by the dramatic industrialization and urbanization and many others.
Genetic engineering has replaced the conventional strategies and has the greater potential to overcome such
challenges. The current review summarized the major challenges encountered by humans and addresses the role of
recombinant DNA technology to overcome aforementioned issues. In line with this, we have detailed the limitations
of genetic engineering and possible future directions for researchers to surmount such limitations through
modification in the current genetic engineering strategies.
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2. Recombinant DNA Technology


Recombinant DNA technology comprises altering genetic material outside an organism to obtain enhanced and
desired characteristics in living organisms or as their products. This technology involves the insertion of DNA
fragments from a variety of sources, having a desirable gene sequence via appropriate vector [12]. Manipulation in
organism's genome is carried out either through the introduction of one or several new genes and regulatory
elements or by decreasing or blocking the expression of endogenous genes through recombining genes and elements
[13]. Enzymatic cleavage is applied to obtain different DNA fragments using restriction endo-nucleases for specific
target sequence DNA sites followed by DNA ligase activity to join the fragments to fix the desired gene in vector.
The vector is then introduced into a host organism, which is grown to produce multiple copies of the incorporated
DNA fragment in culture, and finally clones containing a relevant DNA fragment are selected and harvested [11].
The first recombinant DNA (rDNA) molecules were generated in 1973 by Paul Berg, Herbert Boyer, Annie Chang,
and Stanley Cohen of Stanford University and University of California San Francisco. In 1975, during “The
Asilomar Conference” regulation and safe use of rDNA technology was discussed. Paradoxically to the view of
scientists at the time of Asilomar, the recombinant DNA methods to foster agriculture and drug developments took
longer than anticipated because of unexpected difficulties and barriers to achieve the satisfactory results. However,
since the mid-1980s, the number of products like hormones, vaccines, therapeutic agents, and diagnostic tools has
been developed continually to improve health [13].
A quick approach is offered by recombinant DNA technology to scrutinize the genetic expression of the mutations
that were introduced into eukaryote genes through cloned insulin genes insertion inside a simian virus fragment [3].
In a similar way, tumor growth was inhibited by adenoviral vector that encodes endostain human secretory form
through antiangiogenic effects. Antiangiogenic effect can be enhanced by dl1520 through rescuing replication of
Ad-Endo [14]. Targeted gene disruption has been used to produce antitumor derivatives in other hosts which were
structurally similar for the production pathways [15]. Besides, longer acting therapeutic proteins have been
developed through recombinant DNA technologies; for example, sequences containing additional glycosylation site
are one of the most followed approaches. A new chimeric gene has been developed through this technique which
contains the FSH β-subunit coding sequences and the C-terminal peptide of the hCG β-subunit coding sequences
[16]. Researchers have also developed vectors and combined vectors for gene therapy and genetic modification
approaches. Presently, viral vectors have received immense consideration in clinical settings, some of which have
also been commercialized. In principle, viruses are modified to be safe for clinical purposes. They have several
applications including treatment of severe diseases including cancer either through in vivo or gene therapy (ex vivo),
vaccination, and protein transduction approaches [17]. The production of clinical grade viral vectors improvement
has become possible due to advance manufacturing technologies [18]. At present, due to the severe adverse effects,
retroviral vectors are losing their importance although the viral entities transfer genes quickly and correctly into a
number of species. The simplest nonviral gene delivery system uses “naked” DNA, when injected directly into
certain tissues, particularly muscles, produces significant levels of gene expression with least side effects [19]. More
recently, a P1 vector has been designed to introduce the recombinant DNA into E. coli through electroporation
procedures. This new cloning system is used for establishing 15,000 clone library initially averagely 130−150 kb
pairs insert size. PAC cloning system is considered useful for complex genome analysis and in mapping [20]. The
construction of low copy number vectors, for example, pWSK29, pWKS30, pWSK129, and pWKS130, was carried
out using PCR and recombinant DNA technology. These vectors can also be used for generating unidirectional
deletions with exonuclease, complementation analysis, DNA sequencing, and run-off transcription [21]. A broad
range of applications of recombinant DNA technology has been summarized in Figure 1.

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Figure 1

Illustration of various applications of recombinant DNA technology.

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3. Current Research Progress


Recombinant DNA technology is a fast growing field and researchers around the globe are developing new
approaches, devices, and engineered products for application in different sectors including agriculture, health, and
environment. For example, Lispro (Humalog), in comparison with regular human insulin, is a well effective and fast
acting recombinant insulin [3]. Similarly, Epoetin alfa is a novel and well-recognized recombinant protein that can
be effectively used in curing of anemia [22]. Recombinant hGH was found with a great improvement in treating
children lacking the ability to produce hGH in a required quantity. Clinical testing approval by the FDA in
December 1997 for a recombinant version of the cytokine myeloid progenitor inhibitory factor-1 (MPIF-1) was an
achievement to give recognition to this technology. With its help anticancer drug's side effects can be mitigated
whereas it has the ability to mimic the division of immunologically important cells [23, 24]. The following section
summarizes the most recent developments of recombinant DNA technology.
Clustered regularly interspaced short palindromic repeats (CRISPR), a more recent development of recombinant
DNA technology, has brought out solutions to several problems in different species. This system can be used to
target destruction of genes in human cells. Activation, suppression, addition, and deletion of genes in human's cells,
mice, rats, zebrafish, bacteria, fruit flies, yeast, nematodes, and crops proved the technique a promising one. Mouse
models can be managed for studying human diseases with CRISPR, where individual genes study becomes much
faster and the genes interactions studies become easy by changing multiple genes in cells [25]. The CRISPR of H.
hispanica genome is capable of getting adapted to the nonlytic viruses very efficiently. The associated Cas operon
encodes the interfering Cas3 nucleases and other Cas proteins. The engineering of a strain is required with priming
CRISPR for priming crRNAs production and new spacers acceptance. CRISPR-cas system has to integrate new
spacers into its locus for adaptive immunity generation [26]. Recognition of foreign DNA/RNA and its cleavage is a
controlled process in sequence-specific manner. Information related to the intruder's genetic material is stored by the
host system with the help of photo-spacer incorporation into the CRISPR system [27]. Cas9t (gene editing tool)
represents DNA endonucleases which use RNA molecules to recognize specific target [28]. Class 2 CRISPR-Cas
system with single protein effectors can be employed for genome editing processes. Dead Cas9 is important for
histone modifying enzyme's recruitment, transcriptional repression, localization of fluorescent protein labels, and
transcriptional activation [29]. Targeting of genes involved in homozygous gene knockouts isolation process is
carried out by CRISPR-induced mutations. In this way, essential genes can be analyzed which in turn can be used
for “potential antifungal targets” exploration [30]. Natural CRISPR-cas immunity exploitation has been used for
generation of strains which are resistant to different types of disruptive viruses [31].
CRISPR-Cas, the only adaptive immune system in prokaryotes, contains genomic locus known as CRISPR having
short repetitive elements and spacers (unique sequences). CRISPR array is preceded by AT-rich leader sequence and
flanked by cas genes which encode Cas proteins [32, 33]. In Escherichia coli cas1 and cas2 catalases promote new
spacers through complex formation. Photo-spacer adjacent motif (PAM) is required for interference and acquisition
because the target sequence selection is not random. The memorization of the invader's sequence starts after
CRISPR array transcription into long precursor crRNA. During the final stages of immunity process, target is
degraded through interference with invaded nucleic acids. Specific recognition prevents the system from self-
targeting [32, 34]. In different species ofSulfolobus, the CRISPR loci contain multiple spacers whose sequence
matches conjugative plasmids significantly while in some cases the conjugative plasmids also contain small
CRISPR loci. Spacer acquisition is affected by active viral DNA replication in Sulfolobusspecies whereas the DNA
breaks formation at replication forks causes the process to be stimulated [35]. According to the above information,
CRISPR-Cas system has obtained a unique position in advanced biological systems because of its tremendous role
in the stability and enhancement of immunity.
Zinc-finger nucleases (ZFNs) and transcription activator-like effector nucleases (TALENs) are chimeric nucleases
composed of programmable, sequence-specific DNA-binding modules linked to a nonspecific DNA cleavage
domain. Therapeutic potential of ZFNs and TALENs is more specified and targeted [25, 36, 37]. Similarly,
recombinant protein fibroblast growth factor (FGF-1) has been developed which functions in inducing the formation
of new blood vessels in myocardium. Its injection (biologic bypass) into a human myocardium cause an increased
blood supply to the heart. Apligraf, an FDA approved product, which serves as a recombinant skin replacer,
specified for the leg ulcer's treatment and DermaGraft, is effective in the treatment of diabetic ulcers [38–40]. After
successful production of insulin from E. colithrough recombinant DNA technology, currently several animals,
notably cattle and pigs, have been selected as insulin producing source, which however, triggered immune
responses. The recombinant human insulin is identical to human porcine insulin and comparatively infrequently
elicits immunogenic responses. Furthermore, it is more affordable and can satisfy medical needs more readily.
Human growth hormone was the first protein expressed in tobacco plants [41, 42]. Besides insulin, several new
drugs related to recombinant DNA technology have undergone developmental improvements and a number of
protein production systems have been developed. Several engineered microbial strains have been developed to carry
out the formulation of drugs [41, 43, 44]. Molecular medicine formation that is specifically based on proteins faces
serious issues including methods and biology of the cells which function to produce medically important compounds
through recombinant DNA techniques. To overcome these obstacles, there is intense need to improve quality and
quantity of medicines based on a molecular phenomenon. Cell factories are considered important in recombinant
DNA technologies, but these needed to be explored with more details and in depth as the conventional factories are
not fulfilling the needs [42]. Similarly, the endothelial growth factor and Notch signaling were used to engineer
oncolytic adenovirus which acts as a breast cancer selective agent for the antagonist's expression. This further,
through tumor angiogenesis disruption acts as anticancer agent. This decreases the total blood vessels numbers and
causes a dramatic change along with the perfused vessels which indicates the improved efficacy against the tumor
and vascular effects [13]. Efforts have been made to modify the influenza virus genome using recombinant DNA
technology for development of vaccines. The modifications are based on engineering of vectors to expression of
foreign genes. In practical, the NS gene of the influenza virus was replaced with foreign gene, commonly
chloramphenicol acetyltransferase gene. Thereafter, the RNA previously recombined is expressed and packaged into
virus particles after transfection with purified influenza A virus in the presence of helper virus. It has been clarified
that 5′ terminal and the 3′ terminal bases are sufficient from influenza A virus RNA to produce signals for RNA
replication, RNA transcription, and RNA packaging into influenza virus [15].
The abovementioned new production systems enhance pipelines for development of various vaccines and drugs and
so forth. Production of high quality proteins depends on physiology of a cell and the conditions provided to it. The
expression of proteins becomes retarded if a cell goes under stressful conditions, which may also favor the
production in some cases. Thus, further improvements are required for the better and safe production at genetic and
metabolic levels. Microorganisms are considered the most convenient hosts to produce molecular medicines. These
cells allow the incorporation of foreign genes with less resistant barriers and expression is easily controlled.
Compared to plant and mammalian cells to be taken as hosts, microbial systems provide less complicated machinery
which ultimately enhances the performance and quality of proteins production. The use of common microbial
species, including bacteria and yeasts, is promising but the less common strains have also been observed promising
as being cellular factories to produce recombinant molecular drugs. The increasing demands of drugs and the needs
of quality can be fulfilled with better results if these cellular factories of microorganisms get incorporated into
productive processes of pharmaceuticals (Table 1) [41, 45, 46].

Table 1
Current DNA assembly methods for the synthesis of large DNA molecules. The table has been reproduced from
Nature reviews 14: 781–793, with permission from Nature Publishing Group.

Method Mechanism Overhang Scar Comments Examples of applications


(bp) (bp)

BioBricks Type IIP 8 8 Sequentially assembles small Construction of a functional


restriction numbers of sequences gene expressing enhanced
endonuclease cyan fluorescent protein

BglBricks Type IIP 6 6 Uses a highly efficient and Construction of constitutively


restriction commonly used restriction active gene-expression
Method Mechanism Overhang Scar Comments Examples of applications
(bp) (bp)

endonuclease endonuclease, the devices and chimeric,


recognition sequences of multidomain protein fusions
which are not blocked by the
most common DNA
methylases

Pairwise Type IIS 65 4 Requires attachment tags at Assembly of a 91 kb fragment


selection restriction each end of fragments to act from 1-2 kb fragments
endonuclease as promoters for antibiotic
resistance markers; rapid, as
a liquid culture system is
used

GoldenGate Type IIS 4 0 Allows large-scale assembly; One-step assembly of 2-3


restriction ligations are done in parallel fragments
endonuclease one-step assembly of 2-3
fragment

Overlapping Overlap 0 0 Uses overlapping primers for Usually used for 1–3 kb-long
PCR the PCR amplification of 1– fragments, for example, for
3 kb-long fragments gene cassette construction

CPEC Overlap 20–75 0 Uses a single polymerase for One-step assembly of four
the assembly of multiple 0.17–3.2 kb-long PCR
Method Mechanism Overhang Scar Comments Examples of applications
(bp) (bp)

inserts into any vector in a fragments


one-step reaction in vitro

Gateway Overlap 20 0 Uses a specific recombinase One-step assembly of three


for small-scale assembly 0.8–2.3 kb-long fragments

USER Overlap Up to 708 0 Replaces a thymidine with a One-step assembly of three


uracil in the PCR primers, 0.6–1.5 kb-long fragments
which leaves 3′ overhangs
for cloning after cleaving by
a uracil exonuclease

InFusion Overlap 15 0 Uses an enzyme mix for One-step assembly of three


parallel assembly through a 0.2–3.8 kb-long fragments
“chew-back-and-anneal”
method

SLIC Overlap >30 0 (i) Uses a T4 DNA Generation of a ten-way


polymerase through a chew- assembly of 300–400 bp-long
back method in the absence PCR fragments
of dNTPs
(ii) Uses Recombinase A∗ to
stabilize the annealed
fragments and avoid in vitro
Method Mechanism Overhang Scar Comments Examples of applications
(bp) (bp)

ligation
(iii) Allows the parallel
assembly of several hundred
base-long fragments

Gibson Overlap 40–400 0 Uses enzymatic “cocktails” Assembly of the 1.08


to chew back and anneal for Mb Mycoplasma
the parallel assembly of mycoides JCVI-syn1.0
several kilobase-long genome
fragments

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4. Applications of Recombinant DNA Technology

4.1. Food and Agriculture


Recombinant DNA technology has major uses which made the manufacturing of novel enzymes possible which are
suitable in conditions for specified food-processing. Several important enzymes including lipases and amylases are
available for the specific productions because of their particular roles and applications in food industries. Microbial
strains production is another huge achievement that became possible with the help of recombinant DNA technology.
A number of microbial strains have been developed which produce enzyme through specific engineering for
production of proteases. Certain strains of fungi have been modified so that their ability of producing toxic materials
could be reduced [47]. Lysozymes are the effective agents to get rid of bacteria in food industries. They prevent the
colonization of microbial organisms. It is suitable agent for food items including fruits, vegetables, cheese, and meat
to be stored as it increases their shelf life. The inhibition of food spoiling microorganisms can be carried out through
immobilized lysozyme in polyvinyl alcohol films and cellulose. Lysozyme impregnation of fish skin gelatin gels
increase the shelf life of food products and inhibit different food spoiling bacterial growth [48–50].
Exopolysaccharides ofStaphylococcus and E. coli can be hydrolyzed with the use of DspB which is engineered from
T7. This ability of DspB causes a declination in the bacterial population [50]. Biofilms related to food industries can
be removed by the combining activity of serine proteases and amylases [51]. S. aureus, Salmonella
infantis, Clostridium perfringens, B. cereus, Campylobacter jejuni,L. monocytogenes, Yersinia enterocolitica, and
some other food spoiling microorganisms can be inhibited by glucose oxidase. It is also considered one of the most
important enzymes in food industry to kill wide range of foodborne pathogens [50].
Derivation of recombinant proteins being used as pharmaceuticals came into practice from first plant recently and
many others are through to be used for more production of similar medically important proteins [52].
Wide range of recombinant proteins have been expressed in different plant species to be used as enzymes in
industries, some majorly used proteins in research are proteins present in milk which play a role in nutrition, and
new polymeric proteins are being used in industries and medical field [52]. With the invention of HBV vaccine
production in plants, the oral vaccination concept with edible plants has gained popularity. Plants have been used to
produce several therapeutic protein products, such as casein and lysozyme for improving health of child and
polymers of protein for tissue replacement and surgery. Furthermore, tobacco plants can be engineered genetically to
produce human collagen. High yielding molecular proteins is one of the major tasks under consideration in field of
recombinant DNA technology [52]. Traditional breeding and quantitative trade locus (QTL) analysis assisted in the
identification of a rice variety with protein kinase known as PSTOL1 (phosphorus starvation tolerance1) help in
enhancing root growth in early stages and tolerates phosphorus deficiency [53]. Overexpression of this enzyme
enables root to uptake nutrients in sufficient amount in phosphorus deficient soil which ultimately enhances the
grain yield [54]. Chloroplast genome sequences are important in plant evolution and phylogeny. Rpl22 is considered
to be transferred from chloroplast into nuclear genome. This gene contains a peptide which plays role in delivery of
protein from cytosol to chloroplast. A number of important genes deleted from chloroplast have been observed to be
transferred into nucleus, except ycf1 and ycf2, in order to avoid disruptions in photosynthesis and other necessary
processes. Trans-genesis into chloroplast is considered stable as the nuclear transgenic plants face the problems of
lower expression and transgene escape via pollen. Almost ten thousand copies of transgenes have been incorporated
into the genome of chloroplast [55–57]. Transgene expression is dependent on heterologous regulatory sequences
but independent of cellular control. T7gene10 engineering against salt stress has been found successful but with
lower expression rate into nongreen tissues. γ-tmt gene insertion into chloroplast genome results in multiple layer
formation of the inner chloroplast envelope. Lycopene β-cyclase genes introduction into the plastid genome of
tomato enhances the lycopene conversion into provitamin A [57, 58].
Organ or tissue specific genes identification can be carried out through gene expression profiles. cDNAs with full
lengths are the main resources for expression profiling of genes. 44 K Agilent Oligonucleotide microarray is used
for field grown rice transcriptome analysis. Gene expression fluctuation and transcriptome dynamics can be
predicted by transcriptomic data and meteorological information. These processes and predictions are helpful to
improve crop production and resistance to either environmental or microbial stresses. Resistance to fungal and
bacterial infections can be enhanced by WRKY45 gene in rice which is induced by plant activator benzothiadiazole
that activates innate immune system of plant. The larger grain size can be achieved by inserting qSW5 gene. qSH1
causes the loss of seed shattering by preventing the abscission layer formation. Kala4 gene is responsible for the
black color of rice which makes the rice resistant to attacking pathogens [59, 60]. Genetic modification is needed in
facilitating gene by gene introduction of well-known characters. It allows access to extended range of genes from an
organism. Potato, beans, eggplant, sugar beet, squash, and many other plants are being developed with desirable
characters, for example, tolerance of the herbicide glyphosate, resistance to insects, drought resistance, disease and
salt tolerance. Nitrogen utilization, ripening, and nutritional versatility like characters have also been enhanced [61].

4.2. Health and Diseases


Recombinant DNA technology has wide spectrum of applications in treating diseases and improving health
conditions. The following sections describe the important breakthroughs of recombinant DNA technology for the
improvement of human health:

4.2.1. Gene Therapy


Gene therapy is an advanced technique with therapeutic potential in health services. The first successful report in
field of gene therapy to treat a genetic disease provided a more secure direction toward curing the deadliest genetic
diseases [62, 63]. This strategy shows good response in providing treatment for adenosine deaminase-deficiency
(ADA-SCID), which is a primary immunodeficiency. At the beginning of this technology, several challenges
including maintenance of patients on PEGylated ADA (PEG-ADA) during gene therapy and the targeting of gene
transfer to T-lymphocytes were the reasons for unsuccessful results [64, 65]. However, later on successful results
were obtained by targeting haematopoietic stem cells (HSCs) by using an improved gene transfer protocol and a
myeloablative conditioning regime [66].
Adrenoleukodystrophy (X-ALD) and X-linked disorder are is possible through the expression of specific genes
transferred by lentiviral vector, based on HIV-1 [67]. X-ALD protein expression indicates that gene-correction of
true HSCs was achieved successfully. The use of lentiviral vector was made successful for the first time to treat
genetic human disease [68]. Metastatic melanoma was treated through immunotherapy by enhancing the specific
proteins expression during 2006. This success in the field of health sciences opened up new doors to extend the
research to treat serious death causing diseases through immunotherapy [69]. Highly sustained levels of cells that
were engineered for tumor recognition in blood using a retrovirus encoding a T-cell receptor in two patients up to 1
year after infusion resulted in regression of metastatic melanoma lesions. This strategy was later used to treat
patients with metastatic synovial cell carcinoma [70]. Autologous T-cells were genetically modified to express a
Chimeric Antigen Receptors (CAR) with specificity for the B-cell antigen CD19 for the treatment of chronic
lymphocytic leukemia. Genetically modified cells undergo selective expansion for diseases such as SCID-X1 and
ADA-SCID as a consequence of in vivo selection conferred by the disease pathophysiology despite the correction of
only a modest number of progenitors. Combination of gene and drug therapy's potential has recently been
highlighted in a trial seeking to confer chemoprotection on human HSCs during chemotherapy with alkylating
agents for glioblastoma [71].
Gene transfer to a small number of cells at anatomically discrete sites is a targeted strategy that has the potential to
confer therapeutic benefit. It showed impressive results for incurable autosomal recessive dystrophies such as
congenital blindness and Leber congenital amaurosis (LCA). Swiss–German phase I/II gene therapy clinical trial
aimed to treat chronic granulomatous disease in April 2006 that came up with success [72]. Mobilized CD34+ cells
isolated from peripheral blood were retrovirally transduced and infused into the patient where two-thirds of the
patients showed clear benefit from this treatment. After the treatment silencing of the transgene as a result of
methylation of the viral promoter caused the severity of infection that leaded to the death of patient [73].
Many different cancers including lung, gynecological, skin, urological, neurological, and gastrointestinal tumors, as
well as hematological malignancies and pediatric tumors, have been targeted through gene therapy. Inserting tumor
suppressor genes to immunotherapy, oncolytic virotherapy and gene directed enzyme prodrug therapy are different
strategies that have been used to treat different types of cancers. The p53, a commonly transferred tumor suppressor
gene, is a key player in cancer treating efforts. In some of the strategies, p53 gene transfer is combined with
chemotherapy or radiotherapy. The most important strategies that have been employed until now are vaccination
with tumor cells engineered to express immunostimulatory molecules, vaccination with recombinant viral vectors
encoding tumor antigens and vaccination with host cells engineered to express tumor antigens [19]. New fiber
chimeric oncolytic adenoviruses vectors (Ad5/35-EGFP) offer an affective new anticancer agent for the better cure
of hepatocellular carcinoma. A demonstration of these vectors through proper assaying was significant for
transduction improvement and more progeny of the virus were produced in HCC. A higher level of transgenic
expression was mediated and an enhanced antitumor effect was observed on in vitro HCC cells while keeping the
normal cells protected against cytotoxicity. Tumor growth was also inhibited by utilizing this technology [74].
Cancer gene therapy has become more advanced and its efficacy has been improved in recent years [75].
Treatment of cardiovascular diseases by gene therapy is an important strategy in health care science. In
cardiovascular field, gene therapy will provide a new avenue for therapeutic angiogenesis, myocardial protection,
regeneration and repair, prevention of restenosis following angioplasty, prevention of bypass graft failure, and risk-
factor management. Mutation in gene encoding WASP, a protein regulating the cytoskeleton, causes Wiskott-
Aldrich Syndrome (inherited immunodeficiency). Its treatment requires stem cells transplantation; in case matched
donors are unavailable the treatment is carried out through infusion of autologous HSPCs modified ex vivo by gene
therapy [76]. Metastatic cancer can be regressed through immunotherapy based on the adoptive transfer of gene-
engineered T-cells. Accurate targeting of antigens expressed by tumors and the associated vasculature and the
successful use of gene engineering to retarget T-cells before their transfer into the patient are mainly focused on in
this therapy [77]. Cancer cells often make themselves almost “invisible” to the immune system and its
microenvironment suppresses T-cells survival and migration but genetic engineering of T-cells is the solution to
these challenges. T-cells in cancer patients can be modified by recombining the genes responsible for cancer-
specific antigens recognition, resistance to immunosuppression, and extending survival and facilitating migration to
tumors [78]. Fusion between the genes echinoderm microtubule-associated protein like 4 (EML4) and anaplastic
lymphoma kinase (ALK) is generated by an inversion on the short arm of chromosome confers sensitivity to ALK
inhibitors. Vial-mediated delivery of the CRISPR/Cas9 system to somatic cells of adult animals induces specific
chromosomal rearrangements [79].
Wnt signaling is one of the key oncogenic pathways in multiple cancers. Targeting the Wnt pathway in cancer is an
attractive therapeutic approach, where LGK974 potently inhibits Wnt signaling, has strong efficacy in rodent tumor
models, and is well-tolerated. Head and neck cancer cell lines with loss-of-function mutations in the Notch signaling
pathway have a high response rate to LGK974 [80]. Codon-optimized gene, on the basis of coding sequence of the
influenza virus hemagglutinin gene, was synthesized and cloned into a recombinant modified vaccinia virus Ankara
(MVA). Immunization with MVA-H7-Sh2 viral vector in ferrets proved to be immunogenic as unprotected animals
that were mock vaccinated developed interstitial pneumonia and loss of appetite and weight but vaccination with
MVA-H7-Sh2 protected the animals from severe disease [81]. Viral gene therapy is one of the leading and important
therapies for head and neck cancer. Tumor-associated genes are targeted by viruses, and p53 gene function was
targeted through such therapy at first. Cancer cells can be destroyed by oncolytic viruses through viral replication
and by arming with therapeutic transgenes [82].
High density lipoprotein gene ABCA1 mutation in cells can make the cells be differentiated into macrophages. Gene
knockouts in embryonic stem cells enhance the capability of cells to be differentiated into macrophages and
specifically target the desired pathogens. The allele replacements in this case will assist in studying protein coding
changes and regulatory variants involved in alteration of mRNA transcription and stability in macrophages [83].

4.2.2. Production of Antibodies and Their Derivatives


Plant systems have been recently used for the expression and development of different antibodies and their
derivatives. Most importantly, out of many antibodies and antibody derivatives, seven have reached to the
satisfactory stages of requirements. Transgenic tobacco plants can be used for the production of chimeric secretory
IgA/G known as CaroRx, CaroRx. Oral pathogen responsible for decay of a tooth known as Streptococcus mutants,
can be recognized by this antibody. A monoclonal antibody called T84.66 can affectively function to recognize
antigen carcinoembryonic, which is still considered an affectively characterized marker in cancers of epithelia
[84, 85]. A full-length humanized IgG1 known as anti-HSV and anti-RSV, which can function as the recognizing
agent for herpes simplex virus (HSV)-2-glycoprotein B, has been expressed in transgenic soybean and Chinese
Hamster Ovary (CHO) cells. Antibodies from both sources have been shown to prevent vaginal HSV-2 transmission
in mice after applying topically; if worked similarly in humans it would be considered as inexpensive and affective
prevention against diseases transmitted through sexual interactions [86–88]. 38C13 is scFv antibody based on the
idiotype of malignant B lymphocytes in the well-characterized mouse lymphoma cell line 38C13. Administration of
the antibody to mice resulted in the production of anti-idiotype antibodies that are able to recognize 38C13 cells,
which help to protect the mice against with injected lymphoma cells, is a lethal challenge [89, 90]. Unique markers
recognizing enzymes could be produced through this system, most affectively the surface markers of a malignant B-
cells to work as an effective therapy for non-Hodgkin lymphoma like diseases in human [61]. A monoclonal
antibody known as PIPP is specific for human chorionic gonadotropin recognition. The production of full-length
monoclonal antibody and scFv and diabody derivatives was made possible in plants through transgenesis and
agroinfiltration in tobacco transformed transiently [91]. Testosterone production by stimulated hCG can be inhibited
by each of these antibodies in cells cultured by LEYDIG and uterine weight gain could be delayed in mice, through
which hCG activity is checked. Diagnosis and therapy of tumors can be carried out with the help of antibodies [61].

4.2.3. Investigation of the Drug Metabolism


Complex system of drug metabolizing enzymes involved in the drug metabolism is crucial to be investigated for the
proper efficacy and effects of drugs. Recombinant DNA approaches have recently contributed its role through
heterologous expression, where the enzyme's genetic information is expressed in vitro or in vivo, through the
transfer of gene [92, 93].

4.2.4. Development of Vaccines and Recombinant Hormones


Comparatively conventional vaccines have lower efficacy and specificity than recombinant vaccine. A fear free and
painless technique to transfer adenovirus vectors encoding pathogen antigens is through nasal transfer which is also
a rapid and protection sustaining method against mucosal pathogens. This acts as a drug vaccine where an anti-
influenza state can be induced through a transgene expression in the airway [74].
In vitro production of human follicle-stimulating hormone (FSH) is now possible through recombinant DNA
technology. FSH is considerably a complex heterodimeric protein and specified cell line from eukaryotes has been
selected for its expression. Assisted reproduction treatment through stimulating follicular development is an
achievement of recombinant DNA technology. A large number of patients are being treated through r-FSH. Most
interestingly r-FSH and Luteinizing Hormone (LH) recombination was made successful to enhance the ovulation
and pregnancy [94, 95].

4.2.5. Chinese Medicines


As an important component of alternative medicine, traditional chines medicines play a crucial role in diagnostics
and therapeutics. These medicines associated with theories which are congruent with gene therapy principle up to
some extent. These drugs might be the sources of a carriage of therapeutic genes and as coadministrated drugs.
Transgenic root system has valuable potential for additional genes introduction along with the Ri plasmid. It is
mostly carried with modified genes in A. rhizogenes vector systems to enhance characteristics for specific use. The
cultures became a valuable tool to study the biochemical properties and the gene expression profile of metabolic
pathways. The intermediates and key enzymes involved in the biosynthesis of secondary metabolites can be
elucidated by the turned cultures [96, 97].

4.2.6. Medically Important Compounds in Berries


Improvement in nutritional values of strawberries has been carried through rolC gene. This gene increases the sugar
content and antioxidant activity. Glycosylation of anthocyanins requires two enzymes glycosyl-transferase and
transferase. Some nutrition related genes for different components in strawberry including proanthocyanidin, l-
ascorbate, flavonoid, polyphenols, and flavonoid are important for improving the component of interest through
genetic transformation. In case of raspberry, bHLH and FRUITE4 genes control the anthocyanin components
whereas ERubLRSQ072H02 is related to flavonol. By specific transformation, these genes can enhance the
production and improve the quality. All these mentioned compounds have medical values [98].

4.3. Environment
Genetic engineering has wide applications in solving the environmental issues. The release of genetically engineered
microbes, for example, Pseudomonas fluorescens strain designated HK44, for bioremediation purposes in the field
was first practiced by University of Tennessee and Oak Ridge National Laboratory by working in collaboration
[99, 100]. The engineered strain contained naphthalene catabolic plasmid pUTK21 [101] and a transposon-based
bioluminescence-producing lux gene fused within a promoter that resulted in improved naphthalene degradation and
a coincident bioluminescent response [102]. HK44 serves as a reporter for naphthalene bioavailability and
biodegradation whereas its bioluminescence signaling ability makes it able to be used as an online tool for in situ
monitoring of bioremediation processes [102]. The production of bioluminescent signal is detectable using fiber
optics and photon counting modules [101].

4.3.1. Phytoremediation and Plant Resistance Development


Genetic engineering has been widely used for the detection and absorption of contaminants in drinking water and
other samples. For example, AtPHR1 gene introduction into garden plants Torenia, Petunia, andVerbena changed
their ability for Pi absorption. The AtPHR1 transgenic plants with enhanced Pi absorption ability can possibly
facilitate effective phytoremediation in polluted aquatic environments [103]. A fragment of the AtPHR1 gene was
inserted into binary vector pBinPLUS, which contains an enhanced cauliflower mosaic virus 35S promoter. This
plasmid was named pSPB1898 and was used for transformation [104] in Petunia and Verbena usingAgrobacterium
tumefaciens [105]. AtPHR1 is effective in other plant species, such as Torenia,Petunia, and Verbena [103] but
posttranscriptional modification of the endogenous AtPHR1counterpart might be inhibited by overexpression of
AtPHR1 [103].
Plant metabolism processes identify their importance to use for remediating the environmental pollutants. Some of
the chemicals are not prone to be degraded or digested. TNT is only partially digested in which the nitrogen further
reacts with oxygen to form toxic superoxide. To overcome this issue, the gene responsible for
monodehydroascorbate reductase is knocked out which increases the plant tolerance against TNT. Fine-tuning
enzymatic activity and knockout engineering together enhance the plant responses to toxic metals. Phytochelatin
synthase, a heavy metal binding peptides synthesizing enzyme, revealed a way to enhance tolerance against heavy
metals through enzymatic activity attenuation [106]. Recombinant DNA technology has proven to be effective in
getting rid of arsenic particles that are considered as serious contaminants in soil. PvACR3, a key arsenite [As(III)]
antiporter was expressed inArabidopsis which showed enhanced tolerance to arsenic. Seeds of plants genetically
engineered with PvACR3 can germinate and grow in the presence of higher than normal quantity of arsenate [As(V)]
which are generally lethal to wild-type seeds. Arsenic (As) is reduced by As reductase present in A. thaliana.
Phytochelatins restrict the arsenic movement in root cells and phloem companion cells. OsNramp5 and OsHMA3
represent the transporters to uptake cadmium (Cd) and its retention [107]. In plants, brassino-steroid (BR) is
involved in regulating physiological and developmental processes. Its activity is started with triggering
phosphorylation or dephosphorylation cascade [108].
Recent biotechnological approaches for bioremediation include biosorption, phytostabilization, hyperaccumulation,
dendroremediation, biostimulation, mycoremediation, cyanoremediation, and genoremediation, which majorly
depend on enhancing or preventing specified genes activities. However, the challenges in adopting the successful
technique cannot be ignored [109].

4.3.2. Energy Applications


Several microorganisms, specifically cyanobacteria, mediate hydrogen production, which is environmental friendly
energy source. The specific production is maintained by utilizing the required enzymes properly as these enzymes
play a key role in the product formation. But advanced approaches like genetic engineering, alteration in nutrient
and growth conditions, combined culture, metabolic engineering, and cell-free technology [110–112] have shown
positive results to increase the hydrogen production in cyanobacteria and other biofuels [3, 4]. The
commercialization of this energy source will keep the environment clean which is not possible by using
conventional energy sources releasing CO2and other hazardous chemicals [113]. Also cyanobacteria can be
engineered to make them able to convert of CO2 into reduced fuel compounds. This will make the carbon energy
sources harmless to environment. This approach has been successful for vast range of commodity chemicals, mostly
energy carriers, such as short chain and medium chain alcohols [114].
The conductive biofilms of Geobacter sulfurreducens are potential sources in the field in renewable energy,
bioremediation, and bioelectronics. Deletion of PilZ genes encoding proteins in G. sulfurreducens genome made the
biofilm more active as compared to wild-type. CL-1ln is specified for the strain in which the gene GSU1240 was
deleted. Biofilm production was enhanced along with the production of pili and exopolysaccharide. The electron
acceptor CL-1 produced biofilms that were 6-fold more conductive than wild-type biofilms when they were grown
with electrode. This high fold conductivity lowered the potential losses in microbial fuel cells, decreasing the charge
transfer resistance at the biofilm-anode surface and lowering the formal potential. Potential energy was increased by
lower losses [115].
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5. Current Challenges and Future Prospects


The fact that microbial cells are mostly used in the production of recombinant pharmaceutical indicates that several
obstacles come into their way restricting them from producing functional proteins efficiently but these are handled
with alterations in the cellular systems. Common obstacles which must be dealt with are posttranslational
modifications, cell stress responses activation, and instability of proteolytic activities, low solubility, and resistance
in expressing new genes. Mutations occurring in humans at genetic levels cause deficiencies in proteins production,
which can be altered/treated by incorporation of external genes to fill the gaps and reach the normal levels. The use
of Escherichia coli in recombinant DNA technology acts as a biological framework that allows the producers to
work in controlled ways to technically produce the required molecules through affordable processes [41, 116].
Recombinant DNA research shows great promise in further understanding of yeast biology by making possible the
analysis and manipulation of yeast genes, not only in the test tube but also in yeast cells. Most importantly, it is now
possible to return to yeast by transformation with DNA and cloning the genes using a variety of selectable marker
systems developed for this purpose. These technological advancements have combined to make feasible truly
molecular as well as classical genetic manipulation and analysis in yeast. The biological problems that have been
most effectively addressed by recombinant DNA technology are ones that have the structure and organization of
individual genes as their central issue [117, 118]. Recombinant DNA technology is recently passing thorough
development which has brought tremendous changes in the research lines and opened directions for advanced and
interesting ways of research for biosynthetic pathways though genetic manipulation. Actinomycetes are being used
for pharmaceutical productions, for example, some useful compounds in health sciences and the manipulation of
biosynthetic pathways for a novel drugs generation. These contribute to the production of a major part of
biosynthetic compounds and thus have received immense considerations in recombinant drugs designing. Their
compounds in clinical trials are more applicable as they have shown high level activity against various types of
bacteria and other pathogenic microorganisms. These compounds have also shown antitumor activity and
immunosuppressant activity [119].
Recombinant DNA tech as a tool of gene therapy is a source of prevention and cure against acquired genetic
disorders collectively. DNA vaccines development is a new approach to provide immunity against several diseases.
In this process, the DNA delivered contains genes that code for pathogenic proteins. Human gene therapy is mostly
aimed to treat cancer in clinical trials. Research has focused mainly on high transfection efficacy related to gene
delivery system designing. Transfection for cancer gene therapy with minimal toxicity, such as in case of brain
cancer, breast cancer, lung cancer, and prostate cancer, is still under investigation. Also renal transplantation,
Gaucher disease, hemophilia, Alport syndrome, renal fibrosis, and some other diseases are under consideration for
gene therapy [120].
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6. Conclusions
Recombinant DNA technology is an important development in science that has made the human life much easier. In
recent years, it has advanced strategies for biomedical applications such as cancer treatment, genetic diseases,
diabetes, and several plants disorders especially viral and fungal resistance. The role of recombinant DNA
technology in making environment clean (phytoremediation and microbial remediation) and enhanced resistace of
plants to different adverse acting factors (drought, pests, and salt) has been recognized widely. The improvements it
brought not only in humans but also in plants and microorganisms are very significant. The challenges in improving
the products at gene level sometimes face serious difficulties which are needed to be dealt for the betterment of the
recombinant DNA technology future. In pharmaceuticals, especially, there are serious issues to produce good quality
products as the change brought into a gene is not accepted by the body. Moreover, in case of increasing product it is
not always positive because different factors may interfere to prevent it from being successful. Considering health
issues, the recombinant technology is helping in treating several diseases which cannot be treated in normal
conditions, although the immune responses hinder achieving good results.
Several difficulties are encountered by the genetic engineering strategies which needed to be overcome by more
specific gene enhancement according to the organism's genome. The integration of incoming single-stranded DNA
into the bacterial chromosome would be carried out by a RecA-dependent process. This requires sequence homology
between both entities, the bacterial chromosome and incoming DNA. Stable maintenance and reconstitution of
plasmid could be made easy. The introduction of genetic material from one source into the other is a disaster for
safety and biodiversity. There are several concerns over development of genetically engineered plants and other
products. For example, it is obvious that genetically engineered plants can cross-breed with wild plants, thus
spreading their “engineered” genes into the environment, contaminating our biodiversity. Further, concerns exist
that genetic engineering has dangerous health implications. Thus, further extensive research is required in this field
to overcome such issues and resolve the concerns of common people.

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