Optimal Number of Embryos for Transplantation in Obtaining Genetic-Modified Mice and Goats

Russian Journal of Developmental Biology - The technology of creating genetically modified animals (placental mammals) by microinjection into the pronucleus of a fertilized egg suggests, as one of...     

Autosegregation of enzyme loci in agamospermous progenies of triploid plants of sugar beet (<Emphasis Type="Italic">Beta vulgaris</Emphasis> L.)

The ratios of the phenotypic classes of glucosephosphate isomerase (GPI2) and malate dehydrogenase (MDH1 and MDH2) were studied in agamospermous progenies of triploid sugar beet plants. The ratio of the phenotypic classes of these enzymes corresponds to the calculations based on the assumption of polyteny of chromosomes carrying alleles of the enzyme loci accompanied by the loss of extra copies of the alleles in the first division of a cell entering embryogenesis. An increase in the gene dosage due to polyteny leads to the appearance in the progeny with a definite frequency of alleles that were absent in the original parental plant. The notions of “meiotic autosegregation” and “mitotic autosegregation” characteristic of meiotic and mitotic agamospermy are introduced, as well as the term locus polygenotype characterizing not only the allelic composition and the number of chromosomes, but also the number of chromatids carrying alleles of the marker locus in the cell before its entry into embryogenesis.     

Expression of the enzyme-encoding genes under the influence of colchicine and triton X-100 in nongerminating seeds of sugarbeet (<Emphasis Type="Italic">Beta vulgaris</Emphasis> L.)

The expression of the enzyme-coding genes, controlling glucose-phosphate isomerase (GPI), malate dehydrogenase (MDH), and alcohol dehydrogenase (ADH), was examined in nongerminating seeds of sugarbeet after Triton X-100 (TX-100) and colchicine treatment. Two types of changes revealed included modification of the enzymatic loci expression (change of the isozyme electrophoretic mobility) and inactivation of standard profiles. In the MDH and GPI systems, these processes were found to be associated. Complete isozyme modification was accompanied with the disappearance of standard profiles. In the ADH system, the treatment with TX-100 and colchicine gave rise to two independent processes, including silencing of the Adh1 locus and the appearance of the ADH isozymes with abnormal electrophoretic mobility, which were probably the products of the Adh2 locus. It was suggested that the effect of TX-100 and colchicine on the expression of the enzyme-encoding genes examined depended on the intracellular localization of the encoded enzymes.     

Autosegregation of enzyme loci in agamospermous progenies of triploid plants of sugar beet (Beta vulgaris L.)

The ratios of the phenotypic classes of glucosephosphate isomerase (GP12) and malate dehydrogenase (MDH1 and MDH2) were studied in agamospermous progenies of triploid sugar beet plants. The ratio of the phenotypic classes of these enzymes corresponds to the calculations based on the assumption of polyteny of chromosomes carrying alleles of the enzyme loci accompanied by the loss of extra copies of the alleles in the first division of a cell entering embryogenesis. An increase in the gene dosage due to polyteny leads to the appearance in the progeny with a definite frequency of alleles that were absent in the original parental plant. The notions of meiotic autosegregation and mitotic autosegregation characteristic of meiotic and mitotic agamospermy are introduced, as well as the term locus polygenotype characterizing not only the allelic composition and the number of chromosomes, but also the number of chromatids carrying alleles of the marker locus in the cell before its entry into embryogenesis.     

Polymorphism of PCR profiles and expression of alleles at the locus <Emphasis Type="Italic">Adh1</Emphasis> in agamospermous progeny of sugar beet <Emphasis Type="Italic">Beta vulgaris</Emphasis> L.

A modification of the ISSR amplification method based on using a combination of microsatellite and specific unique primer is proposed and tested. This modification simplifies the detected PCR profiles and allows the examination of DNA regions containing definite genes. Combinations of microsatellite primer Mic2 (5′-gacag-acaga-cagac-a-3′) and one of the primers specific to the Adh1 locus, which controls alcohol dehydrogenase (ADH1) in sugar beet, were employed in this work. The microsatellite primer was used in combination with the following specific primers: Adh1f (5′-agagt-gttgg-agagg-gtgtg-ac-3′) containing the binding site at the fourth exon of gene Adh1, or Adh1r (5′-act(ct)a-cagca-ag(ct)cc-(ct)ac(ct)g-ctcc-3′) that binds to the fifth exon of the same gene. In the agamospermous progeny of individual heterozygous diploid plants of sugar beet with the Adh1-F/Adh1-S genotype, polymorphism of PCR profiles obtained in plants of each of three phenotypic classes (FF, FS, and SS) was detected. Among plants of the progeny from an individual plant that represents the heterozygous phenotypic class FS, differences were revealed not only between the PCR profiles but also in the relative activity of allele isozymes of ADH1.     

Role of polyteny and chromosome-membrane interactions in plant genetic processes

Existing data in the literature on polyteny in plants and in eukaryotes in general, data on the structure of interphase chromosomes and their association with the nuclear membrane are analyzed in the paper. In light of these data, the results of our studies on the ratios of phenotypic classes of marker enzymes in agamospermy (apomictic) progeny of sugar beet are considered. The given data allow to state that chromosome polyteny and their association with nuclear membrane provide not only the realization of hereditary information, but also determine the ratio of genotypes and phenotypes in progeny.     

Effect of triton X-100 on genetic segregation and manifestation of the trait of mono- and dicotyledonousness in sugarbeet (Beta vulgaris L.)

The effect of Triton X-100 (TX-100) on the ratio of phenotypic classes and the expression of morphological traits in the progeny of sugar beet hybrids (No. 12 and No. 2) was investigated. It was shown that the TX-100 exposition on the unopened flower buds of sugar beet plants has different effects on hybrid progenies. In agamospermous progeny of hybrid plant N12ct-4, a significant decrease in the heteroallelic (heterozygous) phenotypic classes of alcohol dehydrogenase (ADH1) fraction was determined. The progeny of hybrid plant N2ct-2 did not express the traits of agamospermous origin, but the appearance of sugar beet seedlings with one cotyledon leaf was detected in it. The obtained results indicate high efficiency of the epimutagenic effect of TX-100 on the early stages of plant ontogenesis.     

Effect of colchicine and Triton X-100 on expression of the enzyme-encoding genes in nongerminating seeds of sugarbeet (Beta vulgaris L.)

The expression of the enzyme-coding genes, controlling glucose-phosphate isomerase (GPI), malate dehydrogenase (MDH), and alcohol dehydrogenase (ADH), was examined in nongerminating seeds of sugarbeet after Triton X-100 (TX-100) and colchicine treatment. Two types of changes revealed included modification of the enzymatic loci expression (change of the isozyme electrophoretic mobility) and inactivation of standard profiles. In the MDH and GPI systems, these processes were found to be associated. Complete isozyme modification was accompanied with the disappearance of standard profiles. In the ADH system, the treatment with TX-100 and colchicine gave rise to two independent processes, including silencing of the Adh1 locus and the appearance of the ADH isozymes with abnormal electrophoretic mobility, which were probably the products of the Adh2 locus. It was suggested that the effect of TX-100 and colchicine on the expression of the enzyme-encoding genes examined depended on the intracellular localization of the encoded enzymes.     

Polymorphism of PCR profiles and expression of alleles at the locus Adh1 in agamospermous progeny of beet root Beta vulgaris L

A modification of the ISSR amplification method based on using a combination of microsatellite and specific unique primer is proposed and tested. This modification simplifies the detected PCR profiles and allows the examination of DNA regions containing definite genes. Combinations of microsatellite primer Mic2 (5'-gacag-acaga-cagac-a-3') and one of the primers specific to the Adh1 locus, which controls alcohol dehydrogenase (ADH1) in sugar beet, were employed in this work. The microsatellite primer was used in combination with the following specific primers: Adh1f (5'-agagt-gttgg-agagg-gtgtg-ac-3') containing the binding site at the fourth exon of gene Adh1, or Adh1r (5'-act(ct)a-cagca-ag(ct)cc-(ct)ac(ct)g-ctcc-3') that binds to the fifth exon of the same gene. In the agamospermous progeny of individual heterozygous diploid plants of sugar beet with the Adh1-F/Adh1-S genotype, polymorphism of PCR profiles obtained in plants of each of three phenotypic classes (FF, FS, and SS) was detected. Among plants of the progeny from an individual plant that represents the heterozygous phenotypic class FS, differences were revealed not only between the PCR profiles but also in the relative activity of allele isozymes of ADH1.     

Using the method of natural samples for studying the variability in sugar beat (<Emphasis Type="Italic">Beta vulgaris</Emphasis> L.) agamospermous seed progeny

The existence of natural genetic and natural mixed samples of seeds was theoretically grounded and experimentally demonstrated. A natural genetic sample is detected when analyzing the seed agamospermous progeny in the sequence coinciding with the sequence of seed setting, i.e., in the order they are located on a branch. The method of natural genetic samples has demonstrated the presence of individual regions with nonrandom distribution of phenotypic classes of agamospermous seeds on the branches of sugar beet plants. This phenotype distribution reflects the state of somatic cells on extended branch regions and the manifestation of this state in seed-bud cells. In turn, the genotype of each seed reflects the state of the seed-bud cell (apozygote) that gave rise to embryo development. We also demonstrated heterogeneity in the ratios of enzyme phenotypes of the seeds set on individual branches, regarding it as a result of the changes arising in somatic tissues at the moment of branching. Analysis of the ratios of seed phenotypes on individual branches of the same plant was named the method of natural mixed samples. The combination of natural genetic and natural mixed samples provides for identifying and analyzing various modes of seed setting (gamospermy and agamospermy) and studying the factors that influence the variability in these processes. We postulated that the nonrandom distribution and ratio of the seed phenotypes on plant branches resulted from a nonrandom endoreduplication of the homologous regions in homologous chromosomes carrying the marker locus alleles.