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5. GENETIKA MIKROORGANISME
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5. GENETIKA MIKROORGANISMEPOKOK BAHASAN5.1 Genes: Structure,
Replication, and Mutation5.2 Genes: Expression and Regulation5.3
Microbial Recombination and Plasmids5.4 Recombinant DNA
Technology5.5 Microbial Genomics
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DNA as the Genetic MaterialNucleic acids Structure DNA
Replication The Genetic CodeGene Structure Mutations and their
Chemical BasisDetection and Isolation of Mutants DNA Repair5.1
Genes: Structure, Replication, and MutationPOKOK BAHASAN
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membahas perbedaan struktur dan komposisi DNA dan RNA membahas
asosiasi protein dengan DNA dan membedakan asosiasi protein-protein
dengan DNA pada DNA prokariotik dan eukariotik. membahas aliran
informasi genetik dari DNA ke RNA ke protein, dan membahas hubungan
di antara urutan DNA dan RNA dan asam amino protein. menjelaskan
replikasi DNA dan proses-proses yang digunakan untuk meminimalkan
kesalahan dan mengoreksi kesalahan-kesalahan tersebut membahas
sifat kode genetik mendefinisikan gen dan menbahas elemen-elemen
pengaturnya, seperti promoter and operator membahas empat bagian
gen bakteri (promoter, leader, daerah penyandi, trailer) membahas
sifat dan penyebab mutasi membahas bermacam-macam mekanisme
perbaikan genetik dan keterbatasannyaKOMPETENSI
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DNA as the Genetic MaterialNucleic acids Structure DNA
Replication The Genetic CodeGene Structure Mutations and their
Chemical BasisDetection and Isolation of Mutants DNA Repair5.1
Genes: Structure, Replication, and MutationPOKOK BAHASAN
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Griffith (1928) demonstrated the phenomenon of transformation:
nonvirulent bacteria could become virulent when live, nonvirulent
bacteria were mixed with dead, virulent bacteriaDNA as the Genetic
Material 5.1 Genes: Structure, Replication, and Mutation
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Avery, MacLeod, and McCarty (1944) demonstrated that the
transforming principle (the material responsible for transformation
to virulence in Griffiths experiments) was DNADNA as the Genetic
Material 5.1 Genes: Structure, Replication, and Mutation
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Hershey and Chase (1952) showed that for the T2 bacteriophage,
only the DNA was needed for infectivity; therefore, they proved
that DNA was the genetic materialDNA as the Genetic Material 5.1
Genes: Structure, Replication, and Mutation
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Over the past decades the relationship between DNA, RNA, and
protein has been established DNA as the Genetic Material DNA is the
genetic material of cells; DNA is precisely copied by a process
called replication A gene is a DNA segment that encodes a
polypeptide, an rRNA, or a tRNA Genes are expressed when the
information they encode is transcribed, forming an RNA molecule
complementary to the original DNA template mRNA molecules direct
the synthesis of proteins; the decoding of the mRNA information
occurs during a process called translation 5.1 Genes: Structure,
Replication, and Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDNA RepairPOKOK BAHASANDNA as Genetic Material5.1 Genes:
Structure, Replication, and Mutation
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DNA Structure DNA is composed of purine and pyrimidine
nucleosides that contain the sugar 2'-deoxyribose and are joined by
phosphodiester bridges Nucleic Acid Structure5.1 Genes: Structure,
Replication, and Mutation
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DNA Structure DNA is usually a double helix consisting of two
chains of nucleotides coiled around each otherNucleic Acid
Structure5.1 Genes: Structure, Replication, and Mutation
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DNA Structure The purine adenine (A) on one strand of DNA is
always paired with the pyrimidine thymine (T) on the other strand,
while the purine guanine (G) is always paired with the pyrimidine
cytosine (C); thus, the two strands are said to be
complementaryNucleic Acid Structure5.1 Genes: Structure,
Replication, and Mutation
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DNA Structure The two strands are not positioned directly
opposite one another; therefore, a major groove and a smaller minor
groove are formed by the double helix backboneNucleic Acid
Structure5.1 Genes: Structure, Replication, and Mutation
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DNA Structure The two polynucleotide chains are antiparallel
(i.e., their sugar-phosphate backbones are oriented in opposite
directions)Nucleic Acid Structure5.1 Genes: Structure, Replication,
and Mutation
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DNA Structure DNA is composed of purine and pyrimidine
nucleosides that contain the sugar 2'-deoxyribose and are joined by
phosphodiester bridges DNA is usually a double helix consisting of
two chains of nucleotides coiled around each other The purine
adenine (A) on one strand of DNA is always paired with the
pyrimidine thymine (T) on the other strand, while the purine
guanine (G) is always paired with the pyrimidine cytosine (C);
thus, the two strands are said to be complementary The two strands
are not positioned directly opposite one another; therefore, a
major groove and a smaller minor groove are formed by the double
helix backbone The two polynucleotide chains are antiparallel
(i.e., their sugar-phosphate backbones are oriented in opposite
directions)Nucleic Acid Structure5.1 Genes: Structure, Replication,
and Mutation
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RNA structure RNA differs from DNA in that it is composed of the
sugar ribose rather than 2'-deoxyriboseNucleic Acid Structure5.1
Genes: Structure, Replication, and Mutation
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RNA structure RNA differs from DNA in that it contains the
pyrimidine uracil (U) instead of thymineNucleic Acid Structure5.1
Genes: Structure, Replication, and Mutation
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RNA structure RNA differs from DNA in that it usually consists
of a single strand that can coil back on itself, rather than two
strands coiled around eachNucleic Acid Structure5.1 Genes:
Structure, Replication, and Mutation
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RNA structure Three different kinds of RNA exist: ribosomal
(rRNA), transfer (tRNA), and messenger (mRNA); they differ from one
another in function, site of synthesis in eucaryotic cells, and
structureNucleic Acid Structure5.1 Genes: Structure, Replication,
and Mutation
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RNA structure RNA differs from DNA in that it is composed of the
sugar ribose rather than 2'-deoxyribose RNA differs from DNA in
that it contains the pyrimidine uracil (U) instead of thymine RNA
differs from DNA in that it usually consists of a single strand
that can coil back on itself, rather than two strands coiled around
each other Three different kinds of RNA exist: ribosomal (rRNA),
transfer (tRNA), and messenger (mRNA); they differ from one another
in function, site of synthesis in eucaryotic cells, and
structureNucleic Acid Structure5.1 Genes: Structure, Replication,
and Mutation
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The organization of DNA in cells In procaryotes, the DNA exists
as a closed circular, supercoiled molecule associated with basic
(histonelike)Nucleic Acid Structure5.1 Genes: Structure,
Replication, and Mutation
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The organization of DNA in cells In eucaryotes, the DNA is more
highly organized; it is associated with basic (histone) proteins
and is coiled into repeating units known as nucleosomesNucleic Acid
Structure5.1 Genes: Structure, Replication, and Mutation
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The organization of DNA in cells In procaryotes, the DNA exists
as a closed circular, supercoiled molecule associated with basic
(histonelike) proteins In eucaryotes, the DNA is more highly
organized; it is associated with basic (histone) proteins and is
coiled into repeating units known as nucleosomesNucleic Acid
Structure5.1 Genes: Structure, Replication, and Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDNA RepairPOKOK BAHASANNucleic Acid Structure 5.1 Genes:
Structure, Replication, and Mutation
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Pattern of DNA synthesis DNA replication is semiconservative:DNA
Replication each strand of DNA is conserved, but the two strands
are separated from each other and serve as templates for the
production of another strand according to the base-pairing rules
discussed earlier5.1 Genes: Structure, Replication, and
Mutation
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Pattern of DNA synthesis Replication forks are the areas of the
DNA molecule where this strand separation occurs and the synthesis
of new DNA takes placeDNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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Pattern of DNA synthesis A replicon consists of an origin of
replication and the DNA that is replicated as a unit from that
originDNA Replication 5.1 Genes: Structure, Replication, and
Mutation
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Pattern of DNA synthesis The bacterial chromosome is usually a
single repliconDNA Replication 5.1 Genes: Structure, Replication,
and Mutation
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Pattern of DNA synthesis Small closed circular DNA molecules,
such as plasmids and some virus genomes, replicate by means of a
rolling-circle mechanismDNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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Pattern of DNA synthesis The large linear DNA molecules of
eucaryotes employ multiple replicons to efficiently replicate the
relatively large molecules within a reasonable time spanDNA
Replication 5.1 Genes: Structure, Replication, and Mutation
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Pattern of DNA synthesis DNA replication is semiconservative:
each strand of DNA is conserved, but the two strands are separated
from each other and serve as templates for the production of
another strand (according to the base-pairing rules discussed
earlier) Replication forks are the areas of the DNA molecule where
this strand separation occurs and the synthesis of new DNA takes
place A replicon consists of an origin of replication and the DNA
that is replicated as a unit from that origin The bacterial
chromosome is usually a single replicon Small closed circular DNA
molecules, such as plasmids and some virus genomes, replicate by
means of a rolling-circle mechanism The large linear DNA molecules
of eucaryotes employ multiple replicons to efficiently replicate
the relatively large molecules within a reasonable time spanDNA
Replication 5.1 Genes: Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DnaA protein
binds to the origin of replication DNA Replication 5.1 Genes:
Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli Helicases
unwind the two strands of DNA and as they do so topoisomerases
(e.g., DNA gyrase) relieve the tension caused by the unwinding
process DNA Replication 5.1 Genes: Structure, Replication, and
Mutation
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Mechanism of DNA replication-as observed in E. coli
Single-stranded DNA binding proteins (SSBs) keep the single strands
apart DNA Replication 5.1 Genes: Structure, Replication, and
Mutation
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Mechanism of DNA replication-as observed in E. coli Primases
synthesize a small RNA molecule (approximately 10 nucleotides) that
will act as a primer for DNA synthesis DNA Replication 5.1 Genes:
Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DNA
polymerase III synthesizes the complementary strand of DNA
according to the base-pairing rules; on one strand (the leading
strand), synthesis is continuous, while on the other (the lagging
strand), a series of fragments are generated by discontinuous
synthesis; a multiprotein complex called a replisome organizes all
of these processesDNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DNA
polymerase I removes the primers and fills the gaps that result
from the RNA deletion DNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DNA ligases
join the DNA fragments to form a complete strand of DNA DNA
Replication 5.1 Genes: Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DNA
replication is extraordinarily complex; at least 30 proteins are
required to replicate the E. coli chromosome DNA Replication 5.1
Genes: Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli The rate of
DNA synthesis is 750 to 1,000 base pairs per second in procaryotes,
and 50 to 100 base pairs per second in eucaryotesDNA Replication
5.1 Genes: Structure, Replication, and Mutation
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Mechanism of DNA replication-as observed in E. coli DnaA protein
binds to the origin of replication Helicases unwind the two strands
of DNA and as they do so topoisomerases (e.g., DNA gyrase) relieve
the tension caused by the unwinding process Single-stranded DNA
binding proteins (SSBs) keep the single strands apart Primases
synthesize a small RNA molecule (approximately 10 nucleotides) that
will act as a primer for DNA synthesis DNA polymerase III
synthesizes the complementary strand of DNA according to the
base-pairing rules; on one strand (the leading strand), synthesis
is continuous, while on the other (the lagging strand), a series of
fragments are generated by discontinuous synthesis; a multiprotein
complex called a replisome organizes all of these processes DNA
polymerase I removes the primers and fills the gaps that result
from the RNA deletion DNA ligases join the DNA fragments to form a
complete strand of DNA DNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDNA RepairPOKOK BAHASANDNA Replication 5.1 Genes: Structure,
Replication, and Mutation
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The Genetic CodeFor polypeptide-coding genes, the DNA base
sequence corresponds to the amino acid sequence of the polypeptide
(colinearity)5.1 Genes: Structure, Replication, and Mutation
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The Genetic CodeEstablishment of the genetic code-each codon
that specifies a particular amino acid must be three bases long for
each of the 20 amino acids to have at least one codon; thus the
genetic code consists of 64 codons 5.1 Genes: Structure,
Replication, and Mutation
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The Genetic CodeOrganization of the code Degeneracy-many amino
acids are encoded by more than one codon Sense codons-61 codons
that specify amino acids Stop (nonsense) codons-three codons (UGA,
UAG, UAA) that do not specify an amino acid, and that are used as
translation (protein synthesis) termination signals
Wobble-describes the somewhat loose base pairing of a tRNA
anticodon to the mRNA codon; wobble eliminates the need for a
unique tRNA for each codon because the first two positions are
sufficient to establish hydrogen bonding between the mRNA and the
aminoacyl-tRNAs5.1 Genes: Structure, Replication, and Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDetection and Isolation of Mutants DNA RepairPOKOK BAHASANThe
Genetic Code5.1 Genes: Structure, Replication, and Mutation
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Gene Structure Gene: a linear sequence of nucleotides that is
within the genomic nucleic acid molecule, and that has a fixed
start point and end point Encodes a polypeptide, a tRNA, or an rRNA
Has controlling elements (e.g., promoters) that regulate expression
of a gene; may be considered as part of the gene itself, or they
may be considered as separate regulatory sequences With some
exceptions, genes are not overlapping The segment that encodes a
single polypeptide is also called a cistron In procaryotes-coding
information is normally continuous although some bacterial genes
are interrupted; in eucaryotes-most genes have coding sequences
(exons) that are interrupted by noncoding sequences (introns) 5.1
Genes: Structure, Replication, and Mutation
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Gene Structure Genes that code for proteins Template strand-the
one strand that contains coding information and directs RNA
synthesis Promoter-a sequence of bases that is usually situated
upstream from the coding region; serves as a recognition/binding
site for RNA polymerase Recognition site-site of initial
association with RNA polymerase (35 bases upstream of transcription
initiation site) Binding site (Pribnow box)-sequence that favors
DNA unwinding before transcription begins (approximately 10 bases
upstream of transcription initiation site) Consensus
sequences-idealized base sequences found most often when comparing
the sequences of different bacteria5.1 Genes: Structure,
Replication, and Mutation
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Gene Structure Genes that code for proteins Leader sequence-a
transcribed sequence that is not translated; contains a consensus
sequence known as the Shine-Dalgarno sequence, which serves as the
recognition site for the ribosome Coding region-the sequence that
begins immediately downstream of the leader sequence; starts with
the template sequence 3'TAC5', which gives rise to mRNA codon
5'AUG3', the first translated codon (specifies N-formylmethionine
in bacteria, methionine in archaea and eucaryotes) Trailer
region-nontranslated region located immediately downstream of the
translation terminator sequence and before the transcription
terminator Regulatory sites-sites where DNA-recognizing regulatory
proteins bind to either stimulate or inhibit gene expression5.1
Genes: Structure, Replication, and Mutation
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Gene Structure Genes that code for tRNA and rRNA tRNA
genes-promoters, leaders, coding regions, and trailer regions are
found; noncoding regions are removed after transcription; more than
one tRNA may be made from a single transcript; the tRNAs are
separated by a noncoding spacer region, which is removed after
transcription rRNA genes-have promoters, leaders, coding regions
and trailer regions; all rRNA molecules are transcribed as a single
large transcript, which is cut up after transcription, yielding the
final rRNA products 5.1 Genes: Structure, Replication, and
Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDNA RepairPOKOK BAHASANGene Structure 5.1 Genes: Structure,
Replication, and Mutation
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Mutations and their Chemical BasisMutation-a stable, heritable
change in the genomic nucleotide sequence5.1 Genes: Structure,
Replication, and Mutation
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Mutations and their Chemical BasisMutations and mutagenesis
Mutations can alter phenotype Morphological mutations-result in
changes in colony or cell morphology Lethal mutations-result in
death of the organism Conditional mutations-are expressed only
under certain environmental conditions Biochemical mutations-result
in changes in the metabolic capabilities of a cellAuxotrophs-cannot
grow on minimal media because they have lost a biosynthetic
capability; require supplements Prototrophs-can grow on minimal
mediaResistance mutations-result in acquired resistance to some
pathogen, chemical, or antibioticMutations can arise spontaneously
or can be induced by a mutagen It is widely held that spontaneous
mutations occur randomly and are then selected; however, one
hypothesis holds that some mutations are directed or adaptive
mutations that may be the result of hypermutation followed by
selection of favorable mutations5.1 Genes: Structure, Replication,
and Mutation
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Mutations and their Chemical BasisSpontaneous mutationsArise
occasionally in all cells without exposure to external agents; they
are often the result of errors in replication Errors in replication
can occur due to tautomeric shifts, which cause base pair
substitutions; other errors can lead to frameshifts
Transition-substitution of one purine for another, or of one
pyrimidine for another Transversion-substitution of a purine for a
pyrimidine or vice versa Frameshift-often the result of the
deletion of nucleotides, which results in an altered codon reading
frame Lesions in the structure of DNA can cause spontaneous
mutations (e.g., loss of a nitrogenous base) Insertion of DNA
segments (e.g., insertion sequences and transposons) can cause
spontaneous mutations 5.1 Genes: Structure, Replication, and
Mutation
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Mutations and their Chemical BasisInduced mutations-caused by
mutagens that damage DNA or alter its chemistry Base analogs are
incorporated into DNA during replication and exhibit base-pairing
properties different from the bases they replace Specific
mispairing occurs when a mutagen changes a bases structure and
thereby alters its pairing characteristics (e.g., alkylating
agents) Intercalating agents, which become inserted between the
stacked bases of the helix, distort the DNA and thus induce single
nucleotide pair insertions or deletions that can lead to
frameshifts Many mutagens (e.g., UV radiation, ionizing radiation,
some carcinogens) can severely damage DNA so that it cannot act as
a replication template; this would be lethal without the repair
mechanisms to restore the DNA; however, the repair mechanisms are
error prone, which also leads to mutations5.1 Genes: Structure,
Replication, and Mutation
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Mutations and their Chemical BasisThe expression of mutations
Forward mutation-a conversion from the most prevalent gene form
(wild type) to a mutant form Reversion-a second mutation that makes
the mutant appear to be a wild type again Back mutation-conversion
of the mutant nucleotide sequence back to the wild type sequence
Suppressor mutation-a reestablishment of the wild type phenotype by
a second mutation that overcomes the effect of the first mutation;
can be in the same gene or a different gene, but does not restore
the original sequenceForward mutation-a conversion from the most
prevalent gene form (wild type) to a mutant form Reversion-a second
mutation that makes the mutant appear to be a wild type again 5.1
Genes: Structure, Replication, and Mutation
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Mutations and their Chemical BasisThe expression of mutations
Point mutations-affect only one base pair and are more common than
large deletions or insertions Silent mutations are alterations of
the base sequence that do not alter the amino acid sequence of the
protein because of code degeneracy Missense mutations are
alterations of the base sequence that result in the incorporation
of a different amino acid in the protein; at the level of protein
function, the effect may range from complete loss of activity, to
no change in activity at all Nonsense mutations are alterations
that produce a translation termination codon, which results in
premature termination of the protein during synthesis; location of
the mutation within the protein will determine the extent of change
in function Frameshift mutations are insertions or deletions of one
or two base pairs that thereby alter the reading frameMutations can
also occur in regulatory sequences and in tRNA and rRNA genes; all
can give observable phenotypes5.1 Genes: Structure, Replication,
and Mutation
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Mutations and their Chemical BasisDetection and Isolation of
Mutants Mutant Detection Visual observation of changes in colony
characteristics Auxotrophic mutants (i.e., those which have lost
the ability to synthesize a particular end product and which
therefore require its presence in the growth medium) can be
detected by replica plating on media with and without the growth
factor; mutants are those growing with the factor but not without
it5.1 Genes: Structure, Replication, and MutationMutant
selection-achieved by finding the environmental condition in which
the mutant will grow but the wild type will not (useful for
isolating auxotrophic revertants and resistance mutants)
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Mutations and their Chemical BasisDetection and Isolation of
Mutants Carcinogenicity testing Many cancer-causing agents
(carcinogens) are also mutagens Tests for mutagenicity are used as
a screen for carcinogenic potential The Ames test is a widely used
mutagenicity test; it detects an increase in reversion of special
strains of Salmonella typhimurium from histidine auxotrophy to
prototrophy after exposure to a potential carcinogen5.1 Genes:
Structure, Replication, and Mutation
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DNA as Genetic MaterialNucleic Acid Structure DNA Replication
The Genetic CodeGene Structure Mutations and their Chemical
BasisDNA RepairPOKOK BAHASANMutations and their Chemical Basis5.1
Genes: Structure, Replication, and Mutation
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5.1 Genes: Structure, Replication, and MutationDNA
RepairExcision repair Corrects damage that causes distortions of
DNA (e.g., thymine dimers, apurinic or apyrimidinic sites, damaged
or unnatural DNA) The damaged area is excised, producing a
single-stranded gap, and then the gap is filled in by DNA
polymerase I and DNA ligase Removal of lesions-reverses damage
without removing and replacing bases; although this process is
error free, it is limited to the repair of certain kinds of damage
(e.g., photoreactivation to remove thymine dimers)
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5.1 Genes: Structure, Replication, and MutationDNA
RepairPostreplication repair-mismatch repair system detects
mismatched base pairs in newly synthesized DNA; these are removed
and replaced by the action of DNA polymerase I and DNA
ligaseRestores DNA that has damage in both strands by recombination
with an undamaged molecule, if available (this frequently occurs in
rapidly dividing cells where there is another copy of the
chromosome not yet parceled out to a daughter cell) SOS repair is a
type of recombination repair; it is used to repair excessive damage
that halts replication; it is an error-prone process that results
in many mutations
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Chapter Web LinksUnderstanding Gene
Testing(http://rex.nci.nih.gov/behindthenews/ugt/ugtframe.htm)
Understanding Gene Testing - tutorial from the National Cancer
Institute
Graphics
Gallery(http://www.accessexcellence.org/AB/GG/#Anchor-Genetics-35326)
Graphics Gallery - click on From Genes to Function for a series of
labeled diagrams with explanations.
Biotech Chronicles(http://www.accessexcellence.org/AB/GG) 5.1
Genes: Structure, Replication, and Mutation
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Konsep-konsep yang akan dipelajari dalam pokok bahasan ini
meliputi: Dua macam asam nukleat, DNA (deoxyribonucleic acid) dan
RNA (ribonucleic acid), berbeda komposisi dan struktur kimianya.
Pada sel prokariotik dan eukariotik, DNA berfungsi sebagai
penyimpan informasi genetik.DNA berasosiasi dengan protein-protein
basa di dalam sel. Pada eukariot, DNA berasosiasi dengan
protein-protein histon khusus, sedangkan pada prokariot, DNA
berasosiasi dengan protein-protein non histone.Gen adalah urutan
nukleotida yang menyandi polipeptida, tRNA, atau rRNA.
Elemen-elemen pengendali seperti promoter dan operator seringkali
dianggap sebagai bagian gen.Sebagian besar gen mempunyai
sekurang-kurangnnya empat bagian utama, masing-masing dengan fungsi
berbeda, promoter, leader, daerah penyandi, and trailers.
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Konsep-konsep yang akan dipelajari dalam pokok bahasan ini
meliputi: Replikasi DNA adalah proses sangat rumit yang melibatkan
sejumlah protein dan tahapan. Replikasi dirancang untuk dapat
berlangsung cepat, tepat, dan dapat diperbaiki ketika kesalahan
terjadi selama proses berlangsung. Informasi genetik terdapat dalam
urutan nukleotida DNA (kadang-kadang RNA). Ketika gen struktural
mengarahkan sintesis polipeptida, masing-masing asam amino disandi
oleh kodon triplet.Mutasi adalah stabil, perubahan yang dapat
diwariskan di dalam gen dan biasanya menghailkan perubahan
fenotipik, Asam nukleat dapat diubah dengan bebeberapa cara, dan
mutasi ini terjadi secara spontan maupun diinduksi oleh mutagen
kimia dan radiasi.Adalah sangat penting untuk mempertahankan urutan
nukleotida selalu konstan, dan mikroorganisme mempunyai beberapa
mekanisme yang dirancang untuk mendeteksi perubahan materi genetik
dan memperbaikinya. Often more than one repair system can correct a
particular type of mutation. Despite these efforts some alterations
remain uncorrected and provide material and opportunity for
evolutionary change.
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menyebutkan the structural and compositional differences between
DNA and RNAmenyebutkan the association of proteins with DNA and
describe the differences in the types of proteins associated with
procaryotic and eucaryotic DNAmengetahui the flow of genetic
information from DNA, to RNA, to protein, and mengetahui the
relationship between the nucleotide sequences of DNA and RNA and
the amino acid sequences of proteinsmengetahui the replication of
DNA and the processes used to minimize errors and correct those
errors which do occurmengetahui the transcription of RNA and
describe the similarities and differences between eucaryotic and
procaryotic RNA transcriptionmengetahui the translation of proteins
and describe the role(s) of the various components required for
this processKOMPETENSI
-
mengetahui the need for metabolic regulation to maintain cell
components at the proper levels and to conserve materials and
energy.kapan on/ofmengetahui regulation by metabolic channeling
(localization) of enzymes and metabolitesmengetahui regulation of
enzyme activity by reversible binding of effector molecules or by
covalent modification of the enzymemengetahui regulation of enzyme
activity by feedback (end product) inhibitionmengetahui regulation
of enzyme synthesis by induction and repression of the genes coding
for a set of related enzymes biomol .. yang penting prinsip-prinsip
tersebutKOMPETENSI
-
menyebutkan the structural and compositional differences between
DNA and RNAmenyebutkan the association of proteins with DNA and
describe the differences in the types of proteins associated with
procaryotic and eucaryotic DNAmengetahui the flow of genetic
information from DNA, to RNA, to protein, and mengetahui the
relationship between the nucleotide sequences of DNA and RNA and
the amino acid sequences of proteinsmengetahui the replication of
DNA and the processes used to minimize errors and correct those
errors which do occurmengetahui the transcription of RNA and
describe the similarities and differences between eucaryotic and
procaryotic RNA transcriptionmengetahui the translation of proteins
and describe the role(s) of the various components required for
this processKOMPETENSI
-
mengetahui the need for metabolic regulation to maintain cell
components at the proper levels and to conserve materials and
energy.kapan on/ofmengetahui regulation by metabolic channeling
(localization) of enzymes and metabolitesmengetahui regulation of
enzyme activity by reversible binding of effector molecules or by
covalent modification of the enzymemengetahui regulation of enzyme
activity by feedback (end product) inhibitionmengetahui regulation
of enzyme synthesis by induction and repression of the genes coding
for a set of related enzymes biomol .. yang penting prinsip-prinsip
tersebutKOMPETENSI
-
5.1 Genes: Structure, Replication, and MutationPokok bahasan ini
menyajikan: konsep dasar genetika molekuler; penyimpanan dan
organisasi informasi genetik molekul DNA, mutagenesis, dan
perbaikannya. peranan mikroorganisme dalam prosedur skrining agen
mutagenik. pembahasan akan ditekankan terutama pada genetika
bakteria
