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artificial gene synthesis

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Imdad Takkar

Gene synthesis allows researchers to chemically synthesize DNA sequences without a template. This involves dividing a desired sequence into short oligonucleotides that are synthesized separately and then assembled. Gene synthesis provides advantages over traditional cloning by allowing customizable sequences that do not exist in nature. It has accelerated research in fields like synthetic biology by providing tools that are faster and cheaper to produce than through cloning.

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Presented by Imdad ali Adnan khan Asia Habib Nouman khan Zahir hussain Usman zeb
 Gene synthesis refers to chemically synthesizing a strand of DNA base-by-base. Unlike DNA replication that occurs in cells or by Polymerase Chain Reaction (PCR), gene synthesis does not require a template strand. Rather, gene synthesis involves the step-wise addition of nucleotides to a single-stranded molecule, which then serves as a template for creation of a complementary strand. Gene synthesis is the fundamental technology upon which the field of synthetic biology has been built
 Artificial gene synthesis is the chemical synthesis of a DNA sequence that represents one or more genes  Artificial gene synthesis provides a method to efficiently produce long stretches of natural and non-natural nucleic acid sequences, broadening the scope of biological experiments.  Sequences that are hard to isolate from natural sources can be routinely generated in the lab, even entirely non-natural gene sequences can be synthesised.
 it also introduces the possibility of developing genes containing modified nucleotides or even novel base pairs that could allow for the expansion of the genetic code.  Therefore, large-scale low-cost methods of gene synthesis must be readily available to facilitate relevant academic and commercial biological research.
 Any DNA sequence can be synthesized, including sequences that do not exist in nature, or variants on naturally-occurring sequences that would be tedious to produce through site-directed mutagenesis, such as codon-optimized sequences for increased heterologous protein expression. Synthetic DNA can be cloned into expression vectors and used in any protocol that requires natural or recombinant DNA. Synthetic genes are used to study all the diverse biological roles that nucleic acids play, from encoding proteins and regulating gene expression in the nucleus, to mediating cell-cell communication and building biofilms from extracellular DNA.
 Gene synthesis technologies have revolutionized biology research. Scientists are no longer limited to classical methods of manipulating a single gene at a time; they now have the power to design or reprogram entire genomes and cells. We can quickly synthesize newly identified viral genomes to accelerate vaccine development. We can engineer novel enzymes that fight cancer and produce sustainable biofuels. We can improve crop yield and reduce vulnerability to the common pests and plant diseases that endanger food supplies and contribute to global hunger. We can detect and break down environmental pollutants in the soil, air and water. We can build designer metabolic circuits using interchangeable synthetic parts
 We can create synthetic genomes and artificial cells to better understand the basic requirements of life. And life science researchers across many disciplines can do more sophisticated experiments, in less time, on smaller budgets, accelerating advances in healthcare, agriculture, energy, and other fields of human endeavor.
 Methods for de novo chemical synthesis of DNA have been refined over the past 60 years. Synthetic short oligonucleotides (oligos) serve as custom primers and probes for a wide variety of applications. Longer sequences that serve as genes or even whole genomes can be synthesized as well; these sequences are typically produced by synthesizing 40-200 bp oligos and then assembling them in the proper order. Many methods for oligo assembly have been developed that rely upon a DNA polymerase enzyme for PCR-based amplification, a DNA ligase enzyme for ligation of oligos, or enzymes that mediate homologous recombination in vitro or in vivo.
 Most sequences up to 1000 base pairs (1 kb) can be assembled in a standard molecular biology lab, and commercial gene synthesis providers routinely synthesize sequences over 10 kb.
 The history of gene synthesis began in 1955, when Sir Alexander Todd published a chemical method for creating a phosphate link between two thymidine nucleosides, effectively describing the first artificial synthesis of a DNA molecule. The first successful synthesis of an entire gene was reported by Gobind Khorana’s group in 1970; the 77 bp DNA fragment took 5 years to synthesize
 Subsequent improvements in DNA synthesis, sequencing, amplification, and automation have made it possible now to synthesize genes over 1 kb in just a few days, and to synthesize much longer sequences including entire genomes.  Gene synthesis can now be easily and cost- effectively outsourced to commercial providers.  GenScript, a pioneer in gene synthesis, was founded in 2002 and is the largest gene synthesis supplier in the world
 1950: DNA polymerase isolated from E. coli. Arthur Kornberg wins 1957 Nobel Prize.  1955 :First DNA molecule synthesized when two thymidine nucleosides are joined by a phoshate link. Sir Alexander Todd wins 1957 Nobel Prize.  1967: DNA ligase is isolated and characterized by five independent laboratories.  1970: First synthesis of an entire gene, a 77 bp yeast tRNA, by Gobind Khorana's group.
1983; Polymerase chain reaction (PCR) is invented. Kary Mullis wins 1993 Nobel Prize. 1983: Caruthers and Matteucci invent phosphoramidite DNA synthesis. 1989: First automated oligonucleotide synthesizer machines become commercially available. 1990s :Improved assembly methods allow synthesis of increasingly long genes.
2003: First synthesis of an entire viral genome, that of phiX174 bacteriophage 2004:Microchip- and microfluidics-based methods for high-throughput gene synthesis are first published 2008 :First complete synthesis of a bacterial genome 2011: Sc2.0 project launched to build the first synthetic eukaryotic genome
 Gene synthesis can generate recombinant, mutated, or completely novel DNA sequences without a template, simplifying the creation of DNA tools that would be laborious to produce through traditional molecular cloning techniques.  A wide variety of types of sequences can be produced to aid in diverse research applications.  In addition to DNA sequences, RNA and oligos containing modified bases or chimeric DNA- RNA backbones can also be synthesized.
 The de novo chemical synthesis of DNA differs from traditional molecular cloning in that it does not require a template.  Gene synthesis allows researchers to specify a desired sequence and custom-build it directly.  Gene synthesis is frequently far more straightforward, faster, and less costly than using alternative methods of molecular cloning and mutagenesis.
Traditional Molecular Cloning • limited to sequences that appear in nature • codon optimization is not feasible • time- and resource-intensive for end- user Gene Synthesis of Bare DNA Fragments • customizable sequence—no template required • time consuming to verify sequences • lower cost for “quick and dirty” high- content, high-throughput screens Gene Synthesis with Subcloning into a Plasmid Vector • customizable sequence—no template required • uniformly accurate sequences from a clone • easy to verify complete sequence using primers that flank gene insert • fast and cost-effective
 Gene Synthesis forms the foundation of the new field of synthetic biology.  Gene synthesis is also accelerating research in well- established research fields by providing critical advantages over more laborious traditional molecular cloning techniques.  De novo gene synthesis is required when template DNA molecules are not available, such as for codon-optimized sequences.  In addition, it is frequently a cost-effective alternative to traditional molecular cloning techniques, such as when multiple DNA segments are being recombined  The case studies below illustrate the power of customizable design afforded by gene synthesis.
 There are usually two methods used for artificial gene synthesis: 1. Oligonucleotide synthesis : They are chemically synthesized by using phosphoramidites these are protecting groups which prevent their amines ,hydroxyl group and phosphate group from interacting incorrectly .
 A set of individually design oligonucleotide is made on automated solid based synthesizer ,purified and then connected by specific annealing and standerd ligation or polymerase reaction. to improve specificity of olegonuclotide annealing the synthesis step relies on a set of thermostable DNA ligase and polymerase enzymes.
 Multiple research groups are searching for a new third base pair for DNA,In 2012 the Amirican scentists Floyed Romesberg are desinged an un natural base,the two new natural base pairs were named d5SICS And dNam. In 2014 the same team synthesized a stretch of circuler DNA known as plasmid cantaining natural T-A and C-G base pairs along with UBP and inserted into cell of Ecoli that succesfully replicated the UBP through multiple generation.
The basic steps of gene synthesis are :  1. sequence optimization and oligo design  2. oligo synthesis  3. gene assembly  4. sequence verification and error correction  5. preparing synthetic DNA for downstream applications
artificial gene synthesis
 Condon optimization to maximize hetrologous protein expression level  Be sure your sequence does not include restriction enzyme recognition site or other sequences that might interfere with your downstream work flow.
 After finalizing the sequence that will be synthesized, sequence analysis is required to determine the best way to divide the whole gene into fragments that will be synthesized and then assembled.  For very large synthetic genes, you will typically want to divide the complete sequence into chunks of 500-1000 kB to be synthesized separately and assembled later.
 oligos synthesis by phosphoramidites,to ensure that nucleotide assembles in correct way and to prevent growing strand from engaging in undesired reaction during synthesis.it can also prevent un wanted branching.
 for assembling oligos in to complete gene building blocks have been developed and successfully used. for short sequences polymerase based invite assembly method. For long sequences in vivo based recombination methods.
 Sequence mutation must be identified and removed.
 Cloning: synthetic gene must be cloned in to vector. synthetic gene design to include, restriction site, recombination are other flanking sequence.
Major applications of artificial gene synthesis are:
 Synthetic modified viral sequences produce safer, more effective DNA vaccines.13 Diniz et al. report that codon optimization augmented both the immunogenicity and the therapeutic anti-tumor effects induced by a DNA vaccine targeting human papillomavirus (HPV)-induced tumors. At the same time, introducing specific point mutations into a viral sequence, such as the modification of the E7 protein sequence found in HPV, can abolish residual oncogenic effects rendering the vaccine less likely to cause harm.
 A fungal plant pathogen induces host cell transdifferentiation and de novo xylem formation. In order to study Verticillium -induced developmental reprogramming of the vascular tissues of host plants (including the economically important Brassica), Reusche et al. used a synthetic gene construct containing a pathogen-inducible promoter driving expression of a transcription factor fused to a strong repression motif. This study reveals the molecular mechanism by which plants compensate for detrimental vein clearance caused by common fungal pathogens, and suggests a way to enhance drought stress resistance.
 Synthetic mutants reveal a novel mechanism for cancer cell metabolic regulation.By synthesizing mutated pyruvate dehydrogenase (PDH) genes, O’Mahoney et al. demonstrated a novel phosphorylation of PDH by AMP kinase that mediates breast cancer cell adaptation to varying glucose availability in the tumor microenvironment, and identified PDH inhibition as a new potential therapeutic strategy for breast cancer.
 1. it have the abality to safley obtain gene for vaccine research with out need to grow full pathogene.  2. These can optimize protein expression in particular host or to remove non functional segments  3. Synthesis of DNA allows DNA storage.
 4. Artificial Gene synthesis can be used to custimize servis to improve antibody affinity.  5. error free synthatic gene for th protein kinases PKB2,S6K1,PDK1

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artificial gene synthesis

  • 1. Presented by Imdad ali Adnan khan Asia Habib Nouman khan Zahir hussain Usman zeb
  • 2.  Gene synthesis refers to chemically synthesizing a strand of DNA base-by-base. Unlike DNA replication that occurs in cells or by Polymerase Chain Reaction (PCR), gene synthesis does not require a template strand. Rather, gene synthesis involves the step-wise addition of nucleotides to a single-stranded molecule, which then serves as a template for creation of a complementary strand. Gene synthesis is the fundamental technology upon which the field of synthetic biology has been built
  • 3.  Artificial gene synthesis is the chemical synthesis of a DNA sequence that represents one or more genes  Artificial gene synthesis provides a method to efficiently produce long stretches of natural and non-natural nucleic acid sequences, broadening the scope of biological experiments.  Sequences that are hard to isolate from natural sources can be routinely generated in the lab, even entirely non-natural gene sequences can be synthesised.
  • 4.  it also introduces the possibility of developing genes containing modified nucleotides or even novel base pairs that could allow for the expansion of the genetic code.  Therefore, large-scale low-cost methods of gene synthesis must be readily available to facilitate relevant academic and commercial biological research.
  • 5.  Any DNA sequence can be synthesized, including sequences that do not exist in nature, or variants on naturally-occurring sequences that would be tedious to produce through site-directed mutagenesis, such as codon-optimized sequences for increased heterologous protein expression. Synthetic DNA can be cloned into expression vectors and used in any protocol that requires natural or recombinant DNA. Synthetic genes are used to study all the diverse biological roles that nucleic acids play, from encoding proteins and regulating gene expression in the nucleus, to mediating cell-cell communication and building biofilms from extracellular DNA.
  • 6.  Gene synthesis technologies have revolutionized biology research. Scientists are no longer limited to classical methods of manipulating a single gene at a time; they now have the power to design or reprogram entire genomes and cells. We can quickly synthesize newly identified viral genomes to accelerate vaccine development. We can engineer novel enzymes that fight cancer and produce sustainable biofuels. We can improve crop yield and reduce vulnerability to the common pests and plant diseases that endanger food supplies and contribute to global hunger. We can detect and break down environmental pollutants in the soil, air and water. We can build designer metabolic circuits using interchangeable synthetic parts
  • 7.  We can create synthetic genomes and artificial cells to better understand the basic requirements of life. And life science researchers across many disciplines can do more sophisticated experiments, in less time, on smaller budgets, accelerating advances in healthcare, agriculture, energy, and other fields of human endeavor.
  • 8.  Methods for de novo chemical synthesis of DNA have been refined over the past 60 years. Synthetic short oligonucleotides (oligos) serve as custom primers and probes for a wide variety of applications. Longer sequences that serve as genes or even whole genomes can be synthesized as well; these sequences are typically produced by synthesizing 40-200 bp oligos and then assembling them in the proper order. Many methods for oligo assembly have been developed that rely upon a DNA polymerase enzyme for PCR-based amplification, a DNA ligase enzyme for ligation of oligos, or enzymes that mediate homologous recombination in vitro or in vivo.
  • 9.  Most sequences up to 1000 base pairs (1 kb) can be assembled in a standard molecular biology lab, and commercial gene synthesis providers routinely synthesize sequences over 10 kb.
  • 10.  The history of gene synthesis began in 1955, when Sir Alexander Todd published a chemical method for creating a phosphate link between two thymidine nucleosides, effectively describing the first artificial synthesis of a DNA molecule. The first successful synthesis of an entire gene was reported by Gobind Khorana’s group in 1970; the 77 bp DNA fragment took 5 years to synthesize
  • 11.  Subsequent improvements in DNA synthesis, sequencing, amplification, and automation have made it possible now to synthesize genes over 1 kb in just a few days, and to synthesize much longer sequences including entire genomes.  Gene synthesis can now be easily and cost- effectively outsourced to commercial providers.  GenScript, a pioneer in gene synthesis, was founded in 2002 and is the largest gene synthesis supplier in the world
  • 12.  1950: DNA polymerase isolated from E. coli. Arthur Kornberg wins 1957 Nobel Prize.  1955 :First DNA molecule synthesized when two thymidine nucleosides are joined by a phoshate link. Sir Alexander Todd wins 1957 Nobel Prize.  1967: DNA ligase is isolated and characterized by five independent laboratories.  1970: First synthesis of an entire gene, a 77 bp yeast tRNA, by Gobind Khorana's group.
  • 13. 1983; Polymerase chain reaction (PCR) is invented. Kary Mullis wins 1993 Nobel Prize. 1983: Caruthers and Matteucci invent phosphoramidite DNA synthesis. 1989: First automated oligonucleotide synthesizer machines become commercially available. 1990s :Improved assembly methods allow synthesis of increasingly long genes.
  • 14. 2003: First synthesis of an entire viral genome, that of phiX174 bacteriophage 2004:Microchip- and microfluidics-based methods for high-throughput gene synthesis are first published 2008 :First complete synthesis of a bacterial genome 2011: Sc2.0 project launched to build the first synthetic eukaryotic genome
  • 15.  Gene synthesis can generate recombinant, mutated, or completely novel DNA sequences without a template, simplifying the creation of DNA tools that would be laborious to produce through traditional molecular cloning techniques.  A wide variety of types of sequences can be produced to aid in diverse research applications.  In addition to DNA sequences, RNA and oligos containing modified bases or chimeric DNA- RNA backbones can also be synthesized.
  • 16.  The de novo chemical synthesis of DNA differs from traditional molecular cloning in that it does not require a template.  Gene synthesis allows researchers to specify a desired sequence and custom-build it directly.  Gene synthesis is frequently far more straightforward, faster, and less costly than using alternative methods of molecular cloning and mutagenesis.
  • 17. Traditional Molecular Cloning • limited to sequences that appear in nature • codon optimization is not feasible • time- and resource-intensive for end- user Gene Synthesis of Bare DNA Fragments • customizable sequence—no template required • time consuming to verify sequences • lower cost for “quick and dirty” high- content, high-throughput screens Gene Synthesis with Subcloning into a Plasmid Vector • customizable sequence—no template required • uniformly accurate sequences from a clone • easy to verify complete sequence using primers that flank gene insert • fast and cost-effective
  • 18.  Gene Synthesis forms the foundation of the new field of synthetic biology.  Gene synthesis is also accelerating research in well- established research fields by providing critical advantages over more laborious traditional molecular cloning techniques.  De novo gene synthesis is required when template DNA molecules are not available, such as for codon-optimized sequences.  In addition, it is frequently a cost-effective alternative to traditional molecular cloning techniques, such as when multiple DNA segments are being recombined  The case studies below illustrate the power of customizable design afforded by gene synthesis.
  • 19.  There are usually two methods used for artificial gene synthesis: 1. Oligonucleotide synthesis : They are chemically synthesized by using phosphoramidites these are protecting groups which prevent their amines ,hydroxyl group and phosphate group from interacting incorrectly .
  • 20.  A set of individually design oligonucleotide is made on automated solid based synthesizer ,purified and then connected by specific annealing and standerd ligation or polymerase reaction. to improve specificity of olegonuclotide annealing the synthesis step relies on a set of thermostable DNA ligase and polymerase enzymes.
  • 21.  Multiple research groups are searching for a new third base pair for DNA,In 2012 the Amirican scentists Floyed Romesberg are desinged an un natural base,the two new natural base pairs were named d5SICS And dNam. In 2014 the same team synthesized a stretch of circuler DNA known as plasmid cantaining natural T-A and C-G base pairs along with UBP and inserted into cell of Ecoli that succesfully replicated the UBP through multiple generation.
  • 22. The basic steps of gene synthesis are :  1. sequence optimization and oligo design  2. oligo synthesis  3. gene assembly  4. sequence verification and error correction  5. preparing synthetic DNA for downstream applications
  • 24.  Condon optimization to maximize hetrologous protein expression level  Be sure your sequence does not include restriction enzyme recognition site or other sequences that might interfere with your downstream work flow.
  • 25.  After finalizing the sequence that will be synthesized, sequence analysis is required to determine the best way to divide the whole gene into fragments that will be synthesized and then assembled.  For very large synthetic genes, you will typically want to divide the complete sequence into chunks of 500-1000 kB to be synthesized separately and assembled later.
  • 26.  oligos synthesis by phosphoramidites,to ensure that nucleotide assembles in correct way and to prevent growing strand from engaging in undesired reaction during synthesis.it can also prevent un wanted branching.
  • 27.  for assembling oligos in to complete gene building blocks have been developed and successfully used. for short sequences polymerase based invite assembly method. For long sequences in vivo based recombination methods.
  • 28.  Sequence mutation must be identified and removed.
  • 29.  Cloning: synthetic gene must be cloned in to vector. synthetic gene design to include, restriction site, recombination are other flanking sequence.
  • 30. Major applications of artificial gene synthesis are:
  • 31.  Synthetic modified viral sequences produce safer, more effective DNA vaccines.13 Diniz et al. report that codon optimization augmented both the immunogenicity and the therapeutic anti-tumor effects induced by a DNA vaccine targeting human papillomavirus (HPV)-induced tumors. At the same time, introducing specific point mutations into a viral sequence, such as the modification of the E7 protein sequence found in HPV, can abolish residual oncogenic effects rendering the vaccine less likely to cause harm.
  • 32.  A fungal plant pathogen induces host cell transdifferentiation and de novo xylem formation. In order to study Verticillium -induced developmental reprogramming of the vascular tissues of host plants (including the economically important Brassica), Reusche et al. used a synthetic gene construct containing a pathogen-inducible promoter driving expression of a transcription factor fused to a strong repression motif. This study reveals the molecular mechanism by which plants compensate for detrimental vein clearance caused by common fungal pathogens, and suggests a way to enhance drought stress resistance.
  • 33.  Synthetic mutants reveal a novel mechanism for cancer cell metabolic regulation.By synthesizing mutated pyruvate dehydrogenase (PDH) genes, O’Mahoney et al. demonstrated a novel phosphorylation of PDH by AMP kinase that mediates breast cancer cell adaptation to varying glucose availability in the tumor microenvironment, and identified PDH inhibition as a new potential therapeutic strategy for breast cancer.
  • 34.  1. it have the abality to safley obtain gene for vaccine research with out need to grow full pathogene.  2. These can optimize protein expression in particular host or to remove non functional segments  3. Synthesis of DNA allows DNA storage.
  • 35.  4. Artificial Gene synthesis can be used to custimize servis to improve antibody affinity.  5. error free synthatic gene for th protein kinases PKB2,S6K1,PDK1