Your search keyword '"Surin VL"' showing total 64 results

1. The spectrum of beta-thalassemia mutations in Azerbaijan

Author

E. A. Gulieva, Tagiev Af, Plutalov Ov, O. K. Kaboev, Surin Vl, Yu. A. Berlin, A. A. Gol'tsov, R. Sh. Rustamov, Dadasheva Ts, E.I. Schwartz, G. Ya. Solovyev, Luk'ianenko Av, and T. A. Mamedova

Subjects

Genetics, Azerbaijan, Base Sequence, Thalassemia, DNA Mutational Analysis, Molecular Sequence Data, beta-Thalassemia, DNA, Biology, medicine.disease, Globins, Mutation, medicine, Humans, Point Mutation, Child, Frameshift Mutation, Genetics (clinical), Alleles, Sequence Deletion

Published

1993

2. Active spread of β-thalassemia beyond the thalassemia belt: A study on a Russian population.

Author

Shchemeleva E, Salomashkina VV, Selivanova D, Tsvetaeva N, Melikyan A, Doronina L, and Surin VL

Abstract

β-Thalassemia is a disease traditionally associated with thalassemia belt countries. Nonetheless, as global migration intensifies, β-thalassemia-causing variants spread far from their origin. We investigated this process to detect some patterns underlying its course. We analyzed β-thalassemia-causing variants and the origin of 676 unrelated participants in Moscow, the largest city of Russia, far away from the thalassemia belt. Our analyses revealed that modern Russia has one of the broadest spectra of thalassemia-causing variants: 46 different variants, including two novel β 0 variants. Only a small proportion of the reported pathogenic variants likely originated in the resident subpopulation. Almost half of the variants that supposedly had emerged outside the Russian borders have already been assimilated by (were found in) the resident subpopulation. The primary modern source of immigration transferring thalassemia to a nonthalassemic part of Russia is the Caucasus region. We also found traces of ancient migration flows from non-Caucasus countries. Our data indicate that β-thalassemia-causing variants are actively spilling over into resident populations of countries outside thalassemia belt regions. Therefore, viewing thalassemia as a disease exclusive to specific ethnic groups creates a mind trap that can complicate the diagnosis., (© 2024 John Wiley & Sons A/S. Published by John Wiley & Sons Ltd.)

Published

2024

3. Traditional multilocus phylogeny fails to fully resolve Palearctic ground squirrels (Spermophilus) relationships but reveals a new species endemic to West Siberia.

Author

Simonov E, Lopatina NV, Titov SV, Ivanova AD, Brandler OV, Surin VL, Matrosova VA, Dvilis AE, Oreshkova NV, Kapustina SY, Golenishchev FN, and Ermakov OA

Subjects

Animals, Siberia, Phylogeny, Asia, Sciuridae genetics, Genetic Introgression

Abstract

Previous efforts to reconstruct evolutionary history of Palearctic ground squirrels within the genus Spermophilus have primarily relied on a single mitochondrial marker for phylogenetic data. In this study, we present the first phylogeny with comprehensive taxon sampling of Spermophilus via a conventional multilocus approach utilizing five mitochondrial and five nuclear markers. Through application of the multispecies coalescent model, we constructed a species tree revealing four distinct clades that diverged during the Late Miocene. These clades are 1) S. alaschanicus and S. dauricus from East Asia; 2) S. musicus and S. pygmaeus from East Europe and northwestern Central Asia; 3) the subgenus Colobotis found across Central Asia and its adjacent regions and encompassing S. brevicauda, S. erythrogenys, S. fulvus, S. major, S. pallidicauda, S. ralli, S. relictus, S. selevini, and S. vorontsovi sp. nov.; and 4) a Central/Eastern Europe and Asia Minor clade comprising S. citellus, S. taurensis, S. xanthoprymnus, S. suslicus, and S. odessanus. The latter clade lacked strong support owing to uncertainty of taxonomic placement of S. odessanus and S. suslicus. Resolving relationships within the subgenus Colobotis, which radiated rapidly, remains challenging likely because of incomplete lineage sorting and introgressive hybridization. Most of modern Spermophilus species diversified during the Early-Middle Pleistocene (2.2-1.0 million years ago). We propose a revised taxonomic classification for the genus Spermophilus by recognizing 18 species including a newly identified one (S. vorontsovi sp. nov.), which is found only in a limited area in the southeast of West Siberia. Employing genome-wide single-nucleotide polymorphism genotyping, we substantiated the role of the Ob River as a major barrier ensuring robust isolation of this taxon from S. erythrogenys. Despite its inherent limitations, the traditional multilocus approach remains a valuable tool for resolving relationships and can provide important insights into otherwise poorly understood groups. It is imperative to recognize that additional efforts are needed to definitively determine phylogenetic relationships between certain species of Palearctic ground squirrels., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

4. A founder effect in hemophilia A patients from Russian Ural region with a new p.(His634Arg) variant in F8 gene.

Author

Salomashkina VV, Pshenichnikova OS, Perina FG, and Surin VL

Subjects

Founder Effect, Haplotypes, Humans, Introns, Mutation, Missense, Factor VIII genetics, Hemophilia A genetics

Abstract

Hemophilia A is a clotting disease caused by defects in the F8 gene. A lot of them are described and most are unique or have polyphyletic origin. We here study the origin of a pathogenic variant found in a few patients. We sequenced F8 gene for seven hemophilia A patients from the Ural region, Sverdlovskaya oblast, Russia. We constructed haplotypes for them and for 21 hemophilia A patients with other defects from the same area as a control group using four previously described X-chromosome loci associated with F8 gene. We identified a new missense variant p.(His634Arg) in seven apparently unrelated patients with mild hemophilia A from Sverdlovskaya oblast. The haplotype analysis showed that all patients share the same haplotype, absent in the other patients, suggesting a founder effect. The most recent common ancestor for the p.(His634Arg) patients is estimated to exist around the end of XVII century; however, the 95% confidence interval spans from XII to early XX century. The Ural region did not suffer from the recent bottlenecks or isolation. Therefore, the founder effect could be a natural consequence of population structuring in a relatively stable population. We identified a founder effect mutation in hemophilia A, which is a quite rare event for this disease., (Copyright © 2021 Wolters Kluwer Health, Inc. All rights reserved.)

Published

2022

5. [Li-Fraumeni syndrome in adult patients with acute lymphoblastic leukemia].

Author

Zarubina KI, Parovichnikova EN, Surin VL, Pshenichnikova OS, Gavrilina OA, Isinova GA, Troitskaya VV, Sokolov AN, Galtseva IV, Kapranov NM, Davydova JO, Obukhova TN, Nikulina EE, Sudarikov AB, and Savchenko VG

Subjects

Adult, Humans, Genes, p53 genetics, Genetic Predisposition to Disease, Germ-Line Mutation, Li-Fraumeni Syndrome diagnosis, Li-Fraumeni Syndrome genetics, Li-Fraumeni Syndrome therapy, Precursor Cell Lymphoblastic Leukemia-Lymphoma diagnosis, Precursor Cell Lymphoblastic Leukemia-Lymphoma genetics, Precursor Cell Lymphoblastic Leukemia-Lymphoma therapy

Abstract

Background: LiFraumeni syndrome (LFS) is a rare, autosomal dominant, hereditary disorder that is characterized by an increased risk for certain types of cancer, acute lymphoblastic leukemia (ALL), particularly. Germline TP53 mutations are associated with LFS. Genetic counseling and follow-up is essential for patients with LFS and their relatives. Special therapeutic approaches are needed for treatment of oncological disease in these patients. The article presents a series of clinical cases of patients with ALL and SLF, considers general issues of diagnosis and treatment of adult patients with this hereditary genetic syndrome., Aim: Describe clinical observations of patients with acute lymphoblastic leukemia (ALL) and LFS and consider general issues of diagnosis and treatment of adult patients with LFS and ALL., Materials and Methods: TP53 gene mutations were screened using Sanger sequencing in 180 de novo patients with Ph-negative (B- and T-cell) and Ph-positive ALL treated by Russian multicenter protocols (ALL-2009, ALL-2012, ALL-2016) at the National Research Center for Hematology, Moscow, Russia, and at the hematology departments of regional clinics of Russia (multicenter study participants)., Results: TP53 gene mutations were found in 7.8% (n=14) of de novo ALL patients. In patients, whose biological material was available TP53 gene mutational status was determined in non-tumor cells (bone marrow and peripheral blood during remission, bone marrow samples after allogeneic hematopoietic stem cells transplantation and in tissue of non-hematopoietic origin) for discriminating germline mutations. The analysis included 5 patients (out of 14 with TP53 mutations), whose non-tumor biological material was available for research. Germline status was confirmed in 4 out of 5 B-cell ALL (n=3), T-cell ALL (n=1) investigated patients., Conclusion: Practical value of the research is the observation that the greater part of TP53 gene mutations in patients with Ph-negative B-cell ALL are germinal and associated with LFS.

Published

2021

6. [Detection of activating mutations in RAS/RAF/MEK/ERK and JAK/STAT signaling pathways].

Author

Zarubina KI, Parovichnikova EN, Surin VL, Pshenichnikova OS, Gavrilina OA, Isinova GA, Troitskaia VV, Sokolov AN, Gal'tseva IV, Kapranov NM, Davydova IO, Obukhova TN, Sudarikov AB, and Savchenko VG

Subjects

Adult, Female, Humans, Male, Mutation, Prospective Studies, Retrospective Studies, Russia, Mitogen-Activated Protein Kinase Kinases

Abstract

Issue: The study of activating mutations (NRAS,KRAS,FLT3,JAK2,CRLF2genes) of RAS/RAF/MEK/ERK and JAK/STAT signaling pathways in B-cell acute lymphoblastic leukemia (B-ALL) in adult patients which are included in Russian multicenter clinical trials., Materials and Methods: Within the multicenter study there were 119 adult patients included withde novoB-ALL. The study was considered as prospective and retrospective. The group withBCR-ABL1-negative B-ALL consisted of up to 93 patients (45 male and 48 female, at the age of 17 to 59, the median age 31), they were treated according to the protocols ALL-2009, ALL-2016. The median follow-up lasted for 19 months (1119). The group withBCR-ABL1-positive B-ALL with up to 26 patients (10 male and 16 female, at the age of 23 to 78, the median age 34 years) was included in the study as well. The treatment was carried out according to the protocols ALL-2009 and ALL-2012 in combination with tyrosine kinase inhibitors. The median follow-up lasted for 23 months (4120). The molecular analysis of activating mutations inNRAS,KRASgenes (RAS/RAF/MEK/ERK signaling pathway) andJAK2,CRLF2genes (JAK/STAT signaling cascade) was performed via Sanger sequencing. The internal tandem duplications (ITDs) inFLT3gene were studied by fragment analysis. The evaluation of CRLF2 expression was fulfilled via flow cytometry., Results: Activating mutations inNRAS,KRAS,FLT3genes were found in 22 (23.6%) patients withBCR-ABL1-negative B-ALL. In total, 23 mutations were revealed in theNRAS(n=9),KRAS(n=12), andFLT3(n=2) genes, according to statistics that was significantly more frequent than withBCR-ABL1-positive B-ALL, these genes mutations were not identified in patients (p=0.007). The frequency of mutations detection inKRASandNRASgenes in patients withBCR-ABL1-negative B-ALL was comparable as 12.9% (12 of 93) to 9.7% (9 of 93), respectively (p=0.488). One patient was simultaneously revealed 2 mutations in theKRASgene (in codons 13 and 61).FLT3-ITD mutations were detected in 3.5% (2 of 57) cases ofBCR-ABL1-negative B-ALL. In patients withBCR-ABL1-positive B-ALLFLT3-ITD mutations were not assessed. Violations in the JAK/STAT signaling cascade were detected in 4 (4.3%) patients withBCR-ABL1-negative B-ALL. They were represented by the missense mutations ofJAK2gene (n=3) and the overexpression of CRLF2 (n=2); in one patient were detected the overexpression of CRLF2 and a mutation inJAK2gene simultaneously. No mutations were found inCRLF2gene. In patients withBCR-ABL1-positive B-ALL noJAK2mutations were detected. As long as analyzing demographic and clinical laboratory parameters between groups of patients with and without mutations, there were no statistically significant differences obtained. In the analyzed groups of patients, long-term therapy results did not differentiate according to the mutations presence inNRAS,KRAS,FLT3,JAK2genes. Also, substantive differences were not shown in the rate of the negative status achievement of the minimum residual disease between patients with and without activating mutations in the control points of the protocol (on the 70th, 133rd and 190th days)., Conclusion: NRAS,KRAS,FLT3,JAK2activating mutations do not affect the long-term results of the therapy and the rate of the negative status achievement of the minimum residual disease in patients withBCR-ABL1-negative B-ALL treated by the Russian multicenter clinical trials.

Published

2020

7. Clonal Composition of Human Multipotent Mesenchymal Stromal Cells: Application of Genetic Barcodes in Research.

Author

Bigildeev AE, Pilunov AM, Sats NV, Surin VL, Shipounova IN, Petinati NA, Logacheva MD, Fedotova AV, Kasyanov AS, Artyukhov AS, Dashinimaev EB, and Drize NJ

Subjects

Cell Proliferation, Cells, Cultured, Gene Library, Humans, Clonal Evolution genetics, Clone Cells metabolism, DNA Barcoding, Taxonomic, Mesenchymal Stem Cells cytology, Mesenchymal Stem Cells metabolism

Abstract

Clonal composition of human multipotent mesenchymal stromal cells (MMSCs) labeled with lentiviral vectors carrying genetic barcodes was studied. MMSCs were transduced with a cloned library of self-inactivating lentiviral vectors carrying 667 unique barcodes. At each cell culture passage, 120 cells were plated one cell per well in 96-well plates. The efficiency of cloning and labeling of the clonogenic cells was determined. DNA was extracted from the cell-derived colonies, and the barcodes were identified by Sanger sequencing. Also, DNA was extracted from the total MMSC population at each passage to analyze the diversity and representation of barcodes by deep sequencing using the Illumina platform. It was shown that the portion of MMSCs labeled with the lentiviral vectors remained stable in the passaged cells. Because of the high multiplicity of infection, the labeling procedure could decrease the proliferative potential of MMSCs. Identification of barcodes in individual cell clones confirmed the polyclonal character of the MMSC population. Clonal composition of MMSCs changed significantly with the passages due to the depletion of proliferative potential of most cells. Large clones were found at the first passage; at later passages, many small clones with a limited proliferative potential were detected in the population. The results of deep sequencing confirmed changes in the clonal composition of MMSCs. The polyclonal MMSC population contained only a small number of cells with a high proliferative potential, some of which could be stem cells. MMSCs with a high proliferative potential were detected more often in the earliest passages. In this regard, we would recommend to use MMSCs of early passages for regenerative medicine applications based on cell proliferation.

Published

2019

8. Coinheritance of HbD-Punjab/β+-thalassemia (IVSI+5 G-C) in patient with Gilbert's syndrome.

Author

Petrenko AA, Pivnik AV, Kim PP, Demidova EY, Surin VL, Abdullaev AO, Sudarikov AB, Petrova NA, and Maryina SA

Subjects

Amino Acid Substitution, Blood Protein Electrophoresis, Gilbert Disease complications, Homozygote, Humans, Male, Pedigree, Sequence Analysis, DNA, Splenomegaly complications, Splenomegaly surgery, Young Adult, beta-Thalassemia complications, Gilbert Disease genetics, Hemoglobins, Abnormal genetics, beta-Thalassemia genetics

Abstract

Thalassemia and qualitative hemoglobinopathy are hereditary disorders of Hb synthesis that lead to change in the Hb conformation or a decrease in the synthesis of structurally normal Hb, and consequently, to erythron pathology. Many variants of Hb are unstable or have altered affinity for oxygen, and, in heterozygous form can be associated with clinical and hematological manifestations (hemolytic anemia, hypochromic microcytic anemia, erythrocytosis). HbD-Punjab [β121 (GH4) Glu → Gln; HBB: C.364G> C] is variant of Hb carrying the amino acid substitution in the 121 position of β-globin chain. In all cases reported so far, patients with HbD-Punjab/β+-thalassemia (IVSI+5 G-C) combination experienced typical thalassemia with hypochromic microcytosis. HbD-Punjab was detected by electrophoresis from 37 to 94% of total Hb. The article describes rare clinical case of the cohabitation of HbD-Punjab/β+-thalassemia (IVSI+5 G-C) in a patient with homozygous variant of Gilbert's syndrome observed in AS Loginov Moscow Clinical Scientific Center.

Published

2018

9. Literature review and clinical observation of acquired idiopathic hemophilia with a new missense mutation in the factor VIII gene (His2026Arg).

Author

Ershov VI, Gadaev IY, Perina FG, Surin VL, Salomashkina VV, Pshenichnikova OS, and Zozulya NI

Subjects

Factor VIIa therapeutic use, Female, Hemophilia A blood, Hemophilia A drug therapy, Humans, Middle Aged, Prednisolone therapeutic use, Recombinant Proteins therapeutic use, Treatment Outcome, Factor VIII genetics, Hemophilia A genetics, Mutation, Missense

Abstract

The article provides review of possible mechanisms of inhibitor coagulopathies, in particular of acquired hemophilia A. This pathology is an extremely rare disease occurring in 1-2 cases in 1 million per year. In the present study we provide data for two clinical cases of hemophilia A in women. These cases had different development mechanisms, although both women have a newly discovered missense mutation His2026Arg in the VIII factor gene. The matter of main interest is the description of the disease development in the patient with an acquired idiopathic hemophilia A with a possible disease occurrence due to an asymmetric X-chromosome inactivation (lyonization). In this particular case lyonization led to the late manifestation of the hemophilia A carrier's state and development of severe form of the inhibitor-associated acquired hemophilia A. We also discuss therapeutic approaches to these forms of the disease, considering there are no concise protocols for case management due to an extreme rarity of the pathology. Acquainting the clinical personnel working it the different areas of medicine with suchlike inhibitor coagulopathies has a major practical importance.

Published

2018

10. DNA analysis of a 30,000-year-old Urocitellus glacialis from northeastern Siberia reveals phylogenetic relationships between ancient and present-day arctic ground squirrels.

Author

Faerman M, Bar-Gal GK, Boaretto E, Boeskorov GG, Dokuchaev NE, Ermakov OA, Golenishchev FN, Gubin SV, Mintz E, Simonov E, Surin VL, Titov SV, Zanina OG, and Formozov NA

Subjects

Animals, Arctic Regions, Cytochromes b genetics, DNA, Mitochondrial, Evolution, Molecular, Geography, Phylogeography, Siberia, DNA, Ancient, Fossils, Phylogeny, Sciuridae classification, Sciuridae genetics

Abstract

In contrast to the abundant fossil record of arctic ground squirrels, Urocitellus parryii, from eastern Beringia, only a limited number of fossils is known from its western part. In 1946, unnamed GULAG prisoners discovered a nest with three mummified carcasses of arctic ground squirrels in the permafrost sediments of the El'ga river, Yakutia, Russia, that were later attributed to a new species, Citellus (Urocitellus) glacialis Vinogr. To verify this assignment and to explore phylogenetic relationships between ancient and present-day arctic ground squirrels, we performed 14 C dating and ancient DNA analyses of one of the El'ga mummies and four contemporaneous fossils from Duvanny Yar, northeastern Yakutia. Phylogenetic reconstructions, based on complete cytochrome b gene sequences of five Late Pleistocene arctic ground squirrels and those of modern U. parryii from 21 locations across western Beringia, provided no support for earlier proposals that ancient arctic ground squirrels from Siberia constitute a distinct species. In fact, we observed genetic continuity of the glacialis mitochondrial DNA lineage in modern U. parryii of the Kamchatka peninsula. When viewed in a broader geographic perspective, our findings provide new insights into the genetic history of U. parryii in Late Pleistocene Beringia.

Published

2017

11. Investigation of the Mesenchymal Stem Cell Compartment by Means of a Lentiviral Barcode Library.

Author

Bigildeev AE, Cornils K, Aranyossy T, Sats NV, Petinati NA, Shipounova IN, Surin VL, Pshenichnikova OS, Riecken K, Fehse B, and Drize NI

Subjects

Animals, Bone Marrow Cells cytology, Cells, Cultured, Female, Gene Library, Mesenchymal Stem Cells cytology, Mice, Mice, Inbred C57BL, Mice, Inbred CBA, Plasmids genetics, Plasmids metabolism, Polymerase Chain Reaction, Lentivirus genetics, Mesenchymal Stem Cells metabolism

Abstract

The hematopoietic bone marrow microenvironment is formed by proliferation and differentiation of mesenchymal stem cells (MSCs). The MSC compartment has been less studied than the hematopoietic stem cell compartment. To characterize the structure of the MSC compartment, it is necessary to trace the fate of distinct mesenchymal cells. To do so, mesenchymal progenitors need to be marked at the single-cell level. A method for individual marking of normal and cancer stem cells based on genetic "barcodes" has been developed for the last 10 years. Such approach has not yet been applied to MSCs. The aim of this study was to evaluate the possibility of using such barcoding strategy to mark MSCs and their descendants, colony-forming units of fibroblasts (CFU-Fs). Adherent cell layers (ACLs) of murine long-term bone marrow cultures (LTBMCs) were transduced with a lentiviral library with barcodes consisting of 32 + 3 degenerate nucleotides. Infected ACLs were suspended, and CFU-F derived clones were obtained. DNA was isolated from each individual colony, and barcodes were analyzed in marked CFU-F-derived colonies by means of conventional polymerase chain reaction and Sanger sequencing. Barcodes were identified in 154 marked colonies. All barcodes appeared to be unique: there were no two distinct colonies bearing the same barcode. It was shown that ACLs included CFU-Fs with different proliferative potential. MSCs are located higher in the hierarchy of mesenchymal progenitors than CFU-Fs, so the presented data indicate that MSCs proliferate rarely in LTBMCs. A method of stable individual marking and comparing the markers in mesenchymal progenitor cells has been developed in this work. We show for the first time that a barcoded library of lentiviruses is an effective tool for studying stromal progenitor cells.

Published

2016

12. [Mutational Analysis of Hemophilia B in Russia: Molecular-Genetic Study].

Author

Surin VL, Demidova EY, Selivanova DS, Luchinina YA, Salomashkina VV, Pshenichnikova OS, and Likhacheva EA

Subjects

Female, Genetics, Population, Hemophilia B pathology, High-Throughput Nucleotide Sequencing, Humans, Phenotype, Promoter Regions, Genetic, Russia, Sequence Analysis, DNA, DNA Mutational Analysis, Factor IX genetics, Hemophilia B genetics, Mutation genetics

Abstract

Hemophilia B is a hereditary X-linked coagulation disorder. This pathology is caused by various defects in the factor IX gene, which is, being about 34 kb long and consisting of eight exons, localized in the Xq27 locus of the. X-chromosome long arm. Mutations were revealed in 56 unrelated patients with hemophilia B in this study by using direct sequencing of factor IX gene functionally important fragments. Forty-six mutations were found with prevailing missense mutations (n = 30). The rest of the mutations were nonsense (n = 4) and splicing (n = 4) mutations, large deletions (n = 3), microdeletions (n = 2), microinsertions (n = 2), and promoter mutations (n = 1). Eleven of 46 mutations were previously unknown for human populations.

Published

2016

13. [Molecular serological characteristics of weak D antigen types of the Rhesus system].

Author

Golovkina LL, Stremoukhova AG, Pushkina TD, Kalandarov RS, Atroshchenko GV, Vasilyeva MN, Surin VL, Salomashkina VV, Pshenichnikova OS, Miterev GY, Parovichnikova EN, and Savchenko VG

Subjects

Humans, Phenotype, Rh-Hr Blood-Group System genetics, Russia epidemiology, Rh-Hr Blood-Group System classification

Abstract

Aim: to estimate the spread of weak D antigen types of the Rhesus system in the citizens of the Russian Federation and a possibility of serologically identifying these types., Subjects and Methods: The red blood cells and DNA of people with weakened expression of D antigen were investigated using erythrocyte agglutination reaction in salt medium (2 methods); agglutination reaction in the gel columns containing IgM + IgG anti-D antibodies, indirect antiglobulin test with IgG anti-D antibodies (2 methods); polymerase chain reaction to establish the type of weak D., Results: A rhesus phenotype was determined in 5100 people in 2014-2015. The weakened agglutinable properties of red blood cells were detected in 102 (2%) examinees. 63 examinees underwent genotyping to identify the variants of the weak D antigen, which identified 6 weak D types. There were the most common weak D types 3 (n=31 (49.2%)) and weak D type 1 (n=18 (28.6%)), including weak D type 1.1 in one (1.6%) case. The other 4 weak D antigen types were as follows: weak D type 2 (14.3% (n=9)), weak D type 15 (4.8% (n=3)), weak D type 4.2 (DAR) (1.6% (n=1)) and weak D type 6 (1.6% (n=1)). The antiglobulin test in the gel column containing antiglobulin serum was the most sensitive serological assay to identify the weak D antigen. Only a molecular test could establish weak D type 15 in 2 samples of red blood cells with Ccdee and ccdEe phenotypes., Conclusion: The weak D antigen could be serologically identified in 96.8% of cases. When testing for weak D, particular attention should be given to people with the D-negative phenotype who had the C or E antigens. Our investigations conducted for the first time in Russia will be able to improve the immunological safety of red blood cell-containing medium transfusions for patients.

Published

2016

14. [Hereditary afibrinogenemia: A literature review and clinical observations].

Author

Yakovleva EV, Surin VL, Selivanova DS, Sergeeva AM, Gonсharova MV, Demidova EY, Soboleva NP, Makhinya SA, Dezhenkova AV, Likhacheva EA, and Zozulya NI

Subjects

Afibrinogenemia complications, Afibrinogenemia diagnosis, Afibrinogenemia therapy, Consanguinity, Fibrinogen, Hemorrhage etiology, Homozygote, Russia, Afibrinogenemia genetics

Abstract

Afibrinogenemia is a rare congenital coagulopathy that leads to life-threatening bleeding. In afibrinogenemia, plasma fibrinogen levels are less than 0.1 g/L. The clinical manifestations of the disease can be both bleeding and thromboses of different localizations, which is determined by the multifunctional role of fibrinogen in hemostasis. The described cases demonstrate different clinical phenotypes of the disease. In both cases the diagnosis was confirmed by genetic examinations that revealed homozygous mutations in the fibrinogen A genes. The nature of the mutations assumes consanguineous marriages, as confirmed by the results of a genealogical analysis. Fibrinogen preparations are promising in treating afibrinogenemia in Russia.

Published

2016

15. Implications of hybridization, NUMTs, and overlooked diversity for DNA Barcoding of Eurasian ground squirrels.

Author

Ermakov OA, Simonov E, Surin VL, Titov SV, Brandler OV, Ivanova NV, and Borisenko AV

Subjects

Animals, DNA, Mitochondrial genetics, Genetic Variation, Cell Nucleus genetics, DNA Barcoding, Taxonomic, Hybridization, Genetic, Mitochondria genetics, Pseudogenes genetics, Sciuridae classification, Sciuridae genetics

Abstract

The utility of DNA Barcoding for species identification and discovery has catalyzed a concerted effort to build the global reference library; however, many animal groups of economical or conservational importance remain poorly represented. This study aims to contribute DNA barcode records for all ground squirrel species (Xerinae, Sciuridae, Rodentia) inhabiting Eurasia and to test efficiency of this approach for species discrimination. Cytochrome c oxidase subunit 1 (COI) gene sequences were obtained for 97 individuals representing 16 ground squirrel species of which 12 were correctly identified. Taxonomic allocation of some specimens within four species was complicated by geographically restricted mtDNA introgression. Exclusion of individuals with introgressed mtDNA allowed reaching a 91.6% identification success rate. Significant COI divergence (3.5-4.4%) was observed within the most widespread ground squirrel species (Spermophilus erythrogenys, S. pygmaeus, S. suslicus, Urocitellus undulatus), suggesting the presence of cryptic species. A single putative NUMT (nuclear mitochondrial pseudogene) sequence was recovered during molecular analysis; mitochondrial COI from this sample was amplified following re-extraction of DNA. Our data show high discrimination ability of 100 bp COI fragments for Eurasian ground squirrels (84.3%) with no incorrect assessments, underscoring the potential utility of the existing reference librariy for the development of diagnostic 'mini-barcodes'.

Published

2015

16. [Molecular genetic study of acute intermittent porphyria in Russia: mutation analysis and functional polymorphism search in porphobilinogen deaminase gene].

Author

Surin VL, Luchinina IuA, Selivanova DS, Pustovoĭt IaS, Karpova IS, Pivnik AV, Luk'ianenko AV, and Kravchenko SK

Subjects

Alleles, Alternative Splicing genetics, DNA Mutational Analysis methods, Female, Ferrochelatase metabolism, Humans, Male, Penetrance, Porphyria, Acute Intermittent enzymology, Russia, Ferrochelatase genetics, Hydroxymethylbilane Synthase genetics, Mutation, Polymorphism, Single Nucleotide, Porphyria, Acute Intermittent genetics

Abstract

Acute intermittent porphyria (AIP) is an autosomal dominant hereditary disease, caused by partial deficiency of porphobilinogen deaminase (PBGD), one of the key enzymes ofheme biosynthesis. This study describes molecular genetics of AIP in Russia. Mutation analysis of PBGD gene in 70 unrelated patients revealed 47 various genetic defects, 28 of which had not been described previously. Mutations 53delT and Argl 73 Trp (recorded 8 times, in total 23%) proved to be the most common in Russia. Microdeletion 53delThas monophyletic origin and was found only in Russia. Molecular genetic examination of 132 relatives of AIP patients from 40 families revealed 52 latent carriers of the disease. Low (about 10%) AIP penetrance indicates that a mutation in the PBGD gene is an important but not sufficient prerequisite for clinical manifestation of the disease. Modulation of penetrance in erythropoietic protoporphyria by coinheritance of a mutant allele and a functionally defective wild type allele of ferrochetalase gene has been shown previously. We hypothesized that similar mechanism works in AIP. Sequencing of the full length PBGD genes from unrelated AIP patients as well as SN P analysis, and the analysis of abnormal PBGD mRNA splicing showed that in case ofAIP, this hypothesis is not true and some other factors are responsible for the penetrance of this disease.

Published

2010

17. [Maintaining of the morphological specificity and genetic introgression in populations of the great tit Parus major and the Japanese tit P. minor in the middle Amur region].

Author

Fedorov VV, Surin VL, Val'chuk OP, Kapitonova LV, Kerimov AB, and Formozov NA

Subjects

Animals, Base Sequence, Cell Nucleus metabolism, Asia, Eastern, Molecular Sequence Data, Phylogeny, Russia, DNA, Mitochondrial genetics, Genetic Variation, Genetics, Population, Passeriformes genetics

Abstract

The ranges of the great tit Parus major and the Japanese tit P. minor overlap in the middle Amur region, where hybridization of these two species occur. These species have contacted for nearly a century on the western slope of the Malyi Khingan Ridge (the central part of the sympatry zone), but the great tit has colonized territories to the east of the ridge only in the last two decades. The percentage of the P. minor's allele of intron 2 of the mioglobin gene has significantly increased from 8.9% in the west to 27.8% in the east in phenotypically major's populations. Thus, the percentage of foreign mtDNA in P. major populations did not change significantly from west (6.2%, n = 120) to east (3.2%, n = 61). Simultaneous use of two genetic markers (one nuclear and the other mitochondrial) supports our conclusion on strong introgression in the populations of both species, which nevertheless maintain their morphological specificity in the contact zone.

Published

2009

18. Infection of stromal and hemopoietic precursor cells with lentivirus vector in vivo and in vitro.

Author

Nifontova IN, Sats NV, Surin VL, Svinareva DA, Gasparian ME, and Drize NJ

Subjects

Animals, Bone Marrow Cells physiology, Cell Line, Female, Femur cytology, Genetic Vectors genetics, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Hematopoietic Stem Cells physiology, Humans, Lentivirus genetics, Lentivirus Infections metabolism, Mice, Mice, Inbred C57BL, Stromal Cells physiology, Bone Marrow Cells virology, Gene Transfer Techniques, Genetic Vectors metabolism, Hematopoietic Stem Cells virology, Lentivirus metabolism, Stromal Cells virology

Abstract

We developed a method for gene transfer into mesenchymal stromal cells. Lentivirus vector containing green fluorescent protein gene for labeling stromal and hemopoietic precursor cells was obtained using two plasmid sets from different sources. The vector was injected into the femur of mice in vivo and added into culture medium for in vitro infection of the stromal sublayer of long-term bone marrow culture. From 25 to 80% hemopoietic stem cells forming colonies in the spleen were infected with lentivirus vector in vivo and in vitro. Fibroblast colony-forming cells from the femoral bones of mice injected with the lentivirus vector carried no marker gene. The marker gene was detected in differentiated descendants from mesenchymal stem cells (bone cavity cells from the focus of ectopic hemopoiesis formed after implantation of the femoral bone marrow cylinder infected with lentivirus vector under the renal capsule of syngeneic recipient). In in vitro experiments, the marker gene was detected in sublayers of long-term bone marrow cultures infected after preliminary 28-week culturing, when hemopoiesis was completely exhausted. The efficiency of infection of stromal precursor cells depended on the source of lentivirus. The possibility of transfering the target gene into hemopoietic precursor cells in vivo is demonstrated. Stromal precursor cells can incorporate the provirus in vivo and in vitro, but conditions and infection system for effective infection should be thoroughly selected.

Published

2008

19. [New efficient extragenic microsatellite markers for hemophilia A carrier state diagnostics].

Author

Surin VL, Luk'ianenko AV, and Luchinina IuA

Subjects

Base Sequence, Chromosomes, Human, X genetics, Female, Genetic Carrier Screening, Hemophilia A diagnosis, Humans, Male, Molecular Sequence Data, Pedigree, Factor VIII genetics, Genetic Markers, Hemophilia A genetics, Microsatellite Repeats

Abstract

In search of new efficient markers for genetic diagnostics of hemophilia A, two tri-nucleotide microsatellite repeats (STR) at chromosome X loci, which flank coagulation factor VIII gene (F8), namely STR HA472--CTT-repeat, which is localized adjacent to the GAB3 gene 163 bp apart from the 3' end of the F8 gene and STR HA544--repeat (CTT)x(ATT)y located at a distance of 375 bp from the 5' end of the F8 gene were discovered. Detailed analysis using PCR and sequencing has shown that STR HA472 contains two long variable CTT-blocks separated by small spacer CCTCCC. The location of recognition site of restriction endonuclease Mnl1 (CCTC) in the spacer permits to test differentially the polymorphic blocks and thus to increase the analysis informativity. STR HA544 is also represented by two polymorphic blocks (CTT and ATT), for separate amplification of which highly informative PCR amplification assays were elaborated. The study has been done using DNA samples of 212 individuals (125 women) from 48 families with hemophilia A carriers. Our results point to Mendelian inheritance of the markers studied, a high number of allelic variants and high heterozygosity, which was 90% and 100% for HA544 and HA472, respectively. This permitted us to use these data for practical gene diagnostics of the carriers and prenatal diagnostics of hemophilia A. In addition to high informativity STR HA472 and HA544 are highly important for diagnostics as they are located at a shorter distance than other known extragenic polymorphisms of the F8 gene. In contrast to dinucleotide repeats, trinucleotide repeats are readily tested, not requiring high-resolution electrophoretic systems. In addition, they are located on the opposite sites of the F8 gene. This permits to control homologous recombination events in the locus and thus to prevent diagnostic mistakes.

Published

2007

20. [Analysis of the AluI polymorphism in intron 1 of the human coagulation factor VIII gene: a new marker for the hemophilia A carrier detection].

Author

Surin VL, Luk'ianenko AV, and Luchinina IuA

Subjects

Alleles, Female, Gene Frequency, Genetic Linkage, Genetic Markers, Hemophilia A diagnosis, Humans, Male, Pregnancy, Prenatal Diagnosis, Alu Elements genetics, Chromosomes, Human, X genetics, Factor VIII genetics, Hemophilia A genetics, Introns genetics, Polymorphism, Single Nucleotide

Abstract

Frequencies of the CIT SNP alleles at position 2403 of the human coagulation factor VIII gene intron 1, containing the AluI restriction endonuclease recognition site, were examined. Genomic DNA samples for the analysis were obtained from the consulted women and their relatives from the families with hemophilia A. A total of 221 unrelated X chromosomes were studied. The two allelic variants were found with similar frequencies of T(Alu+), 0.53 and C(Alu-), 0.47. The heterozygosity index evaluated as equal to 0.50 was correlated with the experimental heterozygote number. The absence of a tight linkage between the AluI SNP and the widely used in the hemophilia A gene diagnostics HindIII polymorphism (CIT SNP at position 103 of intron 19) was demonstrated. Summarized informativity of these two markers for obligate carriers and for those detected in this study constituted 68% (32 out of 47). At the same time using one of the markers, only 40% (HindIII) and 51% (AluI) of the consulted women were informative. The new marker was used in 13 prenatal DNA diagnostics of hemophilia A. A new deletion polymorphism (del TGA, position 2281-2283 of intron 1) was described in close proximity of the AluI SNP with the frequency of about 0.05. among the five other SNP of the factor VIII gene examined (Bme 18I, intron 1; HpaII, intron 13; MnlI, exon 14; Bst4CI, exon 25; and MseI, exon 26) no effective diagnostic markers were found. Only the MnlI polymorphism could be recommended for limited usage.

Published

2007

21. [Acute porphyrias: problem of primary diagnosis in Russia and CIS countries].

Author

Karpova IV, Pustovoĭt IaS, Luchinina IuA, Surin VL, Luk'ianenko AV, Kravshenko SK, and Kremenetskaia AM

Subjects

Adolescent, Adult, Aminolevulinic Acid metabolism, Diagnosis, Differential, Female, Humans, Hydroxymethylbilane Synthase metabolism, Male, Middle Aged, Porphobilinogen metabolism, Porphyria, Acute Intermittent metabolism, Porphyrins blood, Retrospective Studies, Russia, Spectrophotometry, Mass Screening methods, Porphyria, Acute Intermittent diagnosis

Abstract

Aim: To analyse manifestations and experience in primary screening diagnosis of acute porphyrias which are rarely encountered and little known by general practitioners., Material and Methods: The data on 100 patients with the diagnosis acute porphyria have been analysed. Porphyrin metabolism in differential diagnosis was estimated according to standard techniques., Results: Analysis of primary diagnosis of acute porphyria hepatica in Russia (region-related prevalence, duration of diagnosis, complications because of late pathogenetic treatment) demonstrates the importance of screening diagnosis of acute porphyria at the level of municipal clinics., Conclusion: Early diagnosis prevents severe complications of acute porphyria and reduces cost of examinations in search of accurate diagnosis.

Published

2007

22. [A search for Y-chromosomal species-specific markers and their use for hybridization analysis in ground squirrels].

Author

Ermakov OA, Surin VL, Titov SV, Zborovskiĭ SS, and Formozov NA

Subjects

Animals, Chimera genetics, DNA, Mitochondrial genetics, Female, Genetic Markers genetics, Male, Phylogeny, Random Amplified Polymorphic DNA Technique, Russia, Species Specificity, X Chromosome genetics, Hybridization, Genetic, Sciuridae genetics, Sex-Determining Region Y Protein genetics, Y Chromosome genetics

Abstract

In four ground squirrel species from the Volga region-yellow (Spermophilus fulvus), russet (S. major), little (S. pygmaeus), and speckled (S. suslicus)--four hybridization variants (major/fulvus, major/pygmaeus, major/suslicus, and pygmaeus/suslicus) have been reliably described. Earlier we have shown that populations of S. major from the Volga region were characterized by wide introgression of mtDNA from S. fulvus and S. pygmaeus, which probably, resulted from ancient hybridization. In this study, the same populations were used to analyze the introgression of the Y chromosome, which (unlike mtDNA) is paternally inherited. Three genes, ZfY, SRY, and SmcY were tested as Y-chromosomal candidate markers. It was demonstrated that Y chromosome of ground squirrels lacked the ZfY gene, while its homologous structure, ZfY(X), was presumably linked to the X chromosome. The SRY region examined was rather conservative. In particular, the sequences determined in S. major and S. fulvus were identical, while three out of four substitutions found in S. pygmaeus were located in the coding region. The SmcY gene was found to be the most suitable marker, providing distinguishing of all of the four ground squirrel species by nine nucleotide substitutions. Introgression at the Y chromosome was observed only in two cases: in one S. major individual (out of 51 phenotypically pure animals) caught in the major/fulvus sympatry zone, and in four (one litter) out of fourteen S. fulvus individuals caught in close vicinity of the sympatry zone of these two species. Among 28 S. pymaeus and 9 S. suslicus individuals, no foreign SmcY genes were detected. Two colonies of the "hybrid accumulation" type were examined with eight major/suslicus hybrids analyzed in the first and seventeen major/fulvus hybrids in the second colony. The prevalence of the S. major paternal lineages was observed in both colonies (87.5 and 82.4%, respectively). The data obtained suggest that compared to wide mtDNA introgression, introgression of Y chromosome in the Volga region ground squirrels is statistically significantly less frequent event.

Published

2006

23. [Hemolytic anemia due to anomalous unstable hemoglobin Buenos Aires].

Author

Rumiantseva IuV, Surin VL, Smetanina NS, Pliasunova SA, Blokhina LV, Kolodeĭ SV, and Zhirkova LV

Subjects

Anemia, Hemolytic genetics, Child, DNA analysis, Electrophoresis, Polyacrylamide Gel, Humans, Male, Mutation, Anemia, Hemolytic diagnosis, Hemoglobins, Abnormal genetics

Published

2003

24. [Clinical manifestations of porphyrin metabolism disorders].

Author

Pustovoĭt IaS, Karpova IV, Pivnik AV, Surin VL, Luk'ianenko AV, and Luchinina IuA

Subjects

Acute Disease, Adolescent, Adult, Arginine therapeutic use, Chronic Disease, Female, Heme therapeutic use, Humans, Inosine Diphosphate therapeutic use, Middle Aged, Octreotide therapeutic use, Plasmapheresis, Porphyria, Acute Intermittent diagnosis, Porphyria, Acute Intermittent drug therapy, Porphyria, Acute Intermittent etiology, Porphyria, Acute Intermittent metabolism, Porphyria, Erythropoietic diagnosis, Porphyria, Erythropoietic drug therapy, Porphyria, Erythropoietic etiology, Porphyria, Erythropoietic metabolism, Porphyrias drug therapy, Porphyrias etiology, Porphyrias metabolism, Porphyrias diagnosis, Porphyrins metabolism

Abstract

Aim: To characterize patients with various nosological unities [symbol: see text] of porphyria in accordance with their age, clinical symptoms, provoking factors, therapy and outcome., Material and Methods: Patients with acute intermittent porphyria (43), hereditary coproporphyria (8), variegate porphyria (3), porphyria cutanea tarda (7), hepatoerythropoietic porphyria (1), and hereditary erythropoietic porphyria (2) were studied. One patient was suspected of porphyria caused by deficiency of delta-aminolevulenic acid dehydrogenase., Results: The patients were from the CIS. The overwhelming majority of them were young and middle-aged subjects. Rapid development of the disease and severe neurological symptoms were predominantly observed in patients with acute forms of porphyria., Conclusion: Early diagnosis of porphyrin metabolism disorders makes it possible to decrease abruptly the number of cases leading to severe complications, disability, and fatal outcome. The use of inexpensive methods of screening of porphyrin metabolism disorders provides a promising approach to solving this problem. These methods should be used in municipal hospitals. In addition, asymptomatic carriers of defective gene should be revealed at the preclinical stage using various methods of molecular genetic assay.

Published

2003

25. [Allogenic bone marrow transplantation after reduced intensity conditioning regimens in therapy of patients with hemoblastoses].

Author

Demidova IA, Savchenko VG, Ol'shanskaia IuV, Poreshina LP, Kut'ina RM, Surin VL, Misiurin AV, Domracheva EV, and Parovichnikova EN

Subjects

Adolescent, Adult, Cytogenetic Analysis, Disease-Free Survival, Female, Graft Survival, Humans, Male, Middle Aged, Remission Induction, Transplantation Chimera, Bone Marrow Transplantation mortality, Leukemia, Myelomonocytic, Acute surgery, Transplantation Conditioning methods

Abstract

Aim: To investigate effectiveness of allogenic transplantation of the bone marrow (TBM) in the treatment of hemoblastosis patients from a high risk group, the course of donor bone marrow retention, tolerance and antitumor activity of this therapy., Material and Methods: 11 patients received TBM in low-intensity regimen in Hematological Research Center in 1999-2001. All the patients were from a high risk group. Conditioning was based on the combination of fludarabin with busulfan. The transplanted precursor cells were taken from the bone marrow and/or peripheral donor blood. The retention was controlled by differential agglutination of erythrocytes and amplification of hypervariable sites of DNA. Minimal residual disease was controlled by standard cytogenetical tests, fluorescent in situ hybridization or reverse-transcriptase polymerase chain reaction., Results: All the patients tolerated pretransplantation conditioning well. By chimerism, signs of retention of donor bone marrow on day +30 after TBM were observed in 9 patients of 11. Acute graft versus host reaction developed in 5 patients. This reaction was treated conventionally with methylprednisone and cyclosporin A, in 4 cases with a good effect. A complete remission persists in 5 patients. Mean follow-up lasted for 241 days., Conclusion: Thus, transplantation was successful in 50% patients with an unfavourable prognosis who are still in a complete remission. This suggests efficacy of the above method of treatment.

Published

2003

26. [Study of hybridization in four species of ground squirrels (spermophilus: Rodentia, Sciuridae) by molecular genetic methods].

Author

Ermakov OA, Surin VL, Titov SV, Tagiev AF, Luk'ianenko AV, and Formozov NA

Subjects

Animals, Base Sequence, DNA, Mitochondrial, Founder Effect, Molecular Sequence Data, Polymerase Chain Reaction, Pseudogenes, Random Amplified Polymorphic DNA Technique, Restriction Mapping, Russia, Species Specificity, Tumor Suppressor Protein p53 genetics, Chimera, Genetics, Population, Sciuridae genetics

Abstract

Four species of ground squirrel--yellow (Spermophilus fulvus), russet (S. major), small (S. pygmaeus), and spotted (S. suslicus)--occur in the Volga region. Between S. major and S. pigmaeus, S. major and S. fulvus, and S. major and S. suslicus, sporadic hybridization was reported. Using sequencing and restriction analysis, we have examined the mtDNA C region in 13 yellow, 60 russet, 61 small, 45 spotted ground squirrels, and 9 phenotypic hybrids between these species. It was shown that 43% of S. major individuals had "alien" mitotypes typical of S. fulvus and S. pygmaeus. Alien mitotypes occurred both within and outside sympatric zones. No alien mitotypes were found in 119 animals of the other three species, which suggests that only one parental species (S. major) predominantly participates in backcrosses. Phenotypic hybrids S. fulvus x S. major and S. major x S. pygmaeus) were reliably identified using RAPD-PCR of nuclear DNA. However, we could find no significant traces of hybridization in S. major with alien mitotypes. Analysis of p53 pseudogenes of S. major and S. fulvus that were for the first time described in the present study produced similar results: 59 out of 60 individuals of S. major (including S. major with S. fulvus mitotypes) had only the pseudogene variant specific for S. major. This situation is possible even at low hybridization frequencies (less than 1% according to field observations and 1.4 to 2.7% according to nuclear DNA analysis) if dispersal of S. major from the sympatric zones mainly involved animals that obtained alien mtDNA via backcrossing. The prevalence of animals with alien mitotypes in some S. major populations can be explained by the founder effect. Further studies based on large samples are required for clarifying the discrepancies between mitochondrial and nuclear DNA data.

Published

2002

27. [Three new mutations in the porphobilinogen deaminase gene, detected in acute intermittent porphyria patients from Russia].

Author

Surin VL, Luk'ianenko AV, Karpova IV, Misiurin AV, Pustovot IaS, and Pivnik AV

Subjects

Base Sequence, Codon, DNA Primers, Exons, Heterozygote, Introns, Porphyria, Acute Intermittent enzymology, RNA Splicing, RNA, Messenger genetics, Russia, Sequence Deletion, Hydroxymethylbilane Synthase genetics, Mutation, Porphyria, Acute Intermittent genetics

Abstract

Porphobilinogen deaminase (PBGD) is a key enzyme of the heme biosynthetic pathway. Defects in the PBGD gene lead to an autosomal dominant disease, acute intermittent porphyria (AIP). Almost all AIP patients with rare exceptions are heterozygous for the defective gene. To date, at least 160 different mutations causing AIP are identified. Extensive investigations along this line are conducted in many countries of the world. In Russia these studies had not been hitherto performed. Here we report the results of molecular genetic examination of four Russian patients with AIP diagnosed from clinical symptoms. By direct sequencing of the PBGD gene or the corresponding cDNA, we have detected four mutations, three of which were not previously encountered in the world population. These are TAAG deletion in intron 7 between positions +2 and (IVS7 2-5 delTAAG); T deletion in the initiation codon ATG of exon 3, and the G for C replacement at position -1 of intron 5 (IVS5 as -1 G:C), which disrupts splicing. In addition, in one female patient, a known deletion CT in codon 68 was revealed. In two patients, expression of PBGD gene alleles was significantly disproportional, so that normal mRNA prevailed in one case and mRNA of nonerythroid type in the other. Deletion in intron 7 was easily detectable due to the formation of a heteroduplex fragment with abnormal electrophoretic mobility directly in PCR. This simple heteroduplex analysis allowed us to exclude AIP carriage in son and daughter of a female patient with the genetic defect.

Published

2001

28. [The initial results of detecting mutations in the gene of the porphobilinogen deaminase enzyme in patients with acute intermittent porphyria in Russia].

Author

Pivnik AV, Pustovoĭt IaS, Karpova IV, Surin VL, and Luk'ianenko AV

Subjects

Adult, Base Sequence, Chromosome Deletion, Chromosomes, Human, Pair 11 enzymology, Chromosomes, Human, Pair 11 genetics, Female, Humans, Hydroxymethylbilane Synthase blood, Male, Middle Aged, Molecular Sequence Data, Polymerase Chain Reaction methods, Porphyria, Acute Intermittent enzymology, RNA, Messenger genetics, Russia, Hydroxymethylbilane Synthase genetics, Mutation genetics, Porphyria, Acute Intermittent genetics

Published

2000

29. [New breakpoints of t(9;22) translocation in chronic myeloid leukemia].

Author

Misiurin AV, Surin VL, and Tagiev AF

Subjects

Fusion Proteins, bcr-abl genetics, Genes, abl, Humans, Chromosomes, Human, Pair 22, Chromosomes, Human, Pair 9, Leukemia, Myelogenous, Chronic, BCR-ABL Positive genetics, Translocation, Genetic

Published

1999

30. [Amplification of hypervariable genomic regions for establishment of the type of hematopoiesis in hemoblastosis patients after allogeneic bone marrow transplantation].

Author

Demidova IA, Surin VL, Mendeleeva LP, and Savchenko VG

Subjects

Humans, Polymerase Chain Reaction, Repetitive Sequences, Nucleic Acid, Tissue Donors, Transplantation, Homologous, Blast Crisis therapy, Bone Marrow Transplantation, Genome, Human, Hematopoiesis genetics, Immunoglobulin Variable Region genetics

Abstract

To establish the type of hemopoiesis in 15 patients with hemoblastosis subjected to allogenic bone marrow transplantation, the amplification of four hypervariable human genome loci containing tandem repeats with varying copy numbers (loci ApoB, DX, S52, VWF, and YNZ22) were studied by means of polymerase chain reaction. The sensitivity determined by amplification of DNA mixture in dilutions was 1-2%. Based on the data obtained, various types of hemopoiesis recovery after bone marrow transplantation were determined; in most cases, a complete donor chimerism was revealed; in some patients, mixed chimerism; and in one case, a host type of hemopoiesis was found. An association between hemopoiesis type and further development of the disease was observed.

Published

1997

31. [Molecular systematic of hedgehogs (Erinaceidae, Insectivora) of the northeastern palearctic: testing the new method].

Author

Surin VL, Bannikova AA, Tagiev AF, Osokina AV, and Formozov NA

Subjects

Animals, Arctic Regions, DNA, Hedgehogs classification, Polymerase Chain Reaction, Russia, Species Specificity, Hedgehogs genetics

Published

1997

32. [Polymorphism at codon 117 of the granulocyte-macrophage colony-stimulating factor (GM-CSF) gene].

Author

Tagiev AF, Surin VL, Osokina AV, Luk'ianenko AV, Smirnova OV, Tsetaeva NV, Mikhaĭlova EA, Isaev VG, and Grineva NI

Subjects

Adult, Base Sequence, Humans, Molecular Sequence Data, Mutation, Reference Values, Solubility, Water chemistry, Codon genetics, Granulocyte-Macrophage Colony-Stimulating Factor genetics, Polymorphism, Genetic

Abstract

A T-to-C substitution, replacing a hydrophobic isoleucine residue with a hydrophilic threonine residue in position 100 of a mature protein molecule, was found at codon 117 of the GM-CSF gene. The mutation frequencies were estimated in 51 DNA samples from healthy adult donors and also in 20 samples from patients with different neoplastic myeloid disorders. Almost equal substitution frequencies in patients and normal individuals were observed, suggesting that the defect was not associated with leukemia. Additionally the GM-CSF gene intron 1 sequence was refined.

Published

1995

33. [New polymorphic variants of the gene for human blood coagulation factor IX].

Author

Surin VL, Luk'ianenko AV, Tagiev AF, Smirnova OV, Plutalov OV, and Berlin IuA

Subjects

Base Sequence, Genetic Linkage, Humans, Introns, Molecular Sequence Data, Polymerase Chain Reaction, Repetitive Sequences, Nucleic Acid, X Chromosome, DNA, Satellite genetics, Factor IX genetics, Polymorphism, Genetic

Abstract

The polymorphism of Alu-repeats, which are located in the introns of the human factor IX gene (copies 1-3), was studied. To identify polymorphic variants, direct sequencing of PCR products that contained appropriate repeats was used. In each case, 20 unrelated X chromosomes were studied. A polymorphic Dra I site was found near the 3'-end of Alu copy 3 within the region of the polyA tract. A PCR-based testing system with internal control of restriction hydrolysis was suggested. Testing 81 unrelated X chromosomes revealed that the frequency of the polymorphic Dra I site is 0.23. Taq I polymorphism, which was revealed in Alu copy 4 of factor IX gene in our previous work, was found to be closely linked to Dra I polymorphism. Studies in linkage between different types of polymorphisms of the factor IX gene revealed the presence of a rare polymorphism in intron A that was located within the same minisatellite region as the known polymorphic insertion 50bp/Dde I. However, the size of the insertion in our case was 26 bp. Only one polymorphic variant was found among over 150 unrelated X chromosomes derived from humans from Moscow and its vicinity.

Published

1995

34. [Assessment of the frequency of finding polymorphic alleles of the human X-chromosome locus DXS52 in the Muscovite population].

Author

Kaĭdalova AI, Smirnova OV, Surin VL, and Solov'ev GIa

Subjects

Factor VIII genetics, Female, Genetic Markers, Heterozygote, Humans, Moscow, Alleles, Gene Frequency, Polymorphism, Genetic, X Chromosome

Abstract

The frequency of different polymorphic variants of the multiallelic locus DXS52 (St14) of the human X-chromosome, adjacent to the factor VIII gene, was evaluated by means of PCR for the heterogeneous population of Moscow and Moscow oblast'. It was shown that the heterozygosity index of this polymorphism in the studied population is much lower (0.71) than in Western Europe (0.80-0.85), which can apparently be explained by a higher frequency of the prevailing allele 1690 (0.52 compared to 0.36). Five new St14 alleles were detected during this study. The total informativity of the polymorphic markers St14 and HindIII (intron 19 of the factor VIII gene), which are most commonly used for hemophilia A detection, was evaluated. Among 83 investigated women, only 57 (69%) were heterozygous for at least one of the markers used, which is also much lower than in Western-European populations (90-95%).

Published

1994

35. [A new polymorphism in the human factor IX gene, useful for determining carriers of hemophilia B].

Author

Surin VL, Luk'ianenko AV, Tagiev AF, and Smirnova OV

Subjects

Base Sequence, DNA Primers, Female, Humans, Male, Molecular Sequence Data, Pedigree, Polymerase Chain Reaction, Factor IX genetics, Genetic Carrier Screening, Hemophilia B genetics, Polymorphism, Genetic

Abstract

A new Taq I polymorphism in Alu repeat 4 of the human factor IX gene is reported. This polymorphism is associated with a C-T transition at the 72-bp position of the Alu repeat consensus sequence. A simple PCR system for testing of this structural anomaly, with internal control of restriction hydrolysis, was developed. The frequency of the new polymorphic site and its linkage with other polymorphisms of the factor IX gene were also evaluated. The new polymorphism was used for establishing hemophilia B carriers.

Published

1994

36. [Spectrum of DNA haplotypes and beta-thalassemia mutations linked with them in the Azerbaijan Republic].

Author

Tagiev AF, Surin VL, Luk'ianenko AV, Kulieva EA, Mamedova TA, and Solov'ev GIa

Subjects

Azerbaijan epidemiology, Genetics, Population, Humans, beta-Thalassemia epidemiology, DNA genetics, Genetic Linkage, Haplotypes, Mutation, beta-Thalassemia genetics

Abstract

Haplotyping of the beta-globin gene cluster was performed on DNA samples from 110 Azerbaidzhanian beta-thalassemic patients and their families. During this study, we found 18 different haplotypes and determined the frequency of their occurrence. Nine of these haplotypes have never been observed earlier in the studied population. One of the haplotypes was found only in beta-thalassemia alleles. Several haplotypes were associated with beta-thalassemia mutations found earlier in Azerbaidzhan.

Published

1994

37. [Structure of integrated oncogens E1A and E1B in a malignant line of rat SH2 fibroblasts, transformed by monkey adenovirus SA7 (C8) DNA].

Author

Surin VL, Sats NV, and Tagiev AF

Subjects

Adenoviruses, Simian genetics, Animals, Base Sequence, Blotting, Southern, Cell Line, Transformed, Fibroblasts metabolism, Molecular Sequence Data, Polymerase Chain Reaction, Rats, Adenovirus E1A Proteins genetics, Adenovirus E1B Proteins genetics, Adenoviruses, Simian metabolism, Cell Transformation, Neoplastic genetics, DNA, Viral, Genes, Viral, Oncogenes

Abstract

In this investigation the primary structure of E1A and E1B regions of SA7 (C8) simian adenovirus integrated in malignant SH2 rat cell line was studied. Southern blotting revealed at least two copies of the SA7 oncogene integrated in the SH2 genome. PCR analysis of E1A and E1B regions showed heteroduplex structures, proving the different structure of the integrated copies. The heteroduplex molecules with different electrophoretic mobility were separated, and chains corresponding to different copies were sequenced according to the modified Sanger method. We found that two copies differ mainly in microsatellite regions, in E1A between positions 894-902 (GCG)3/(GCG)4, in E1B between positions 2037-2048 (GCA)3/(GCA)4. It is necessary to stress that all deviations found belong to the coding regions of the SA7 oncogene.

Published

1994

38. [Nucleotide sequence of the E1B area and the adjacent 3'-terminal segment of the E1A oncogene from monkey adenovirus SA7 (C8)].

Author

Sats NV, Surin VL, and Tagiev AF

Subjects

Adenoviruses, Simian genetics, Base Sequence, DNA, Viral, Molecular Sequence Data, Point Mutation, Sequence Homology, Nucleic Acid, Adenovirus E1A Proteins genetics, Adenoviruses, Simian metabolism, Oncogenes

Abstract

The SA7 (C8) simian adenovirus was sequenced from the 1478th to 3194th nucleotide. The region includes the 3'-terminal part of E1A and the major part of the E1B coding region. The sequence obtained was compared with the structure of SA7 (P) DNA previously determined in the region 1-2338, and many differences were found which are nucleotide substitutions, microdeletions and microinsertions. Among point substitutions the most frequent was the C-->T transition in CG pairs known as hot spots of mutations. Differences of our sequence from the previously published one was also revealed.

Published

1994

39. [DNA probes for the alternative splicing region of the 6th exon of the human CSF-1 gene. Polymerase chain reaction and subcloning].

Author

Lanina TP, Aleksandrova NM, Surin VL, Iasenskaia EV, and Grineva NI

Subjects

Base Sequence, Blood Donors, Cloning, Molecular, DNA Probes, Humans, Molecular Sequence Data, Polymerase Chain Reaction, Alternative Splicing, Exons, Hematologic Diseases genetics, Macrophage Colony-Stimulating Factor genetics, Polymorphism, Genetic, RNA, Messenger genetics

Abstract

The DNA probes--pA6-CSF-1 and pA2-CSF-1 for the alternative splicing region of the 6 exon human CSF-1 gene were prepared using PCR and subsequent subcloning in pUC19 plasmid at the XmaI/BamHI sites. Due to the insert sequencing and blotting of human leukocytes DNA, the DNA probes obtained can be useful for screening of mutations in the human CSF-1 gene.

Published

1993

40. [Use of the polymerase chain reaction to detect beta-thalassemia mutations in heterozygous carriers from Azerbaijan while performing prenatal DNA-diagnosis].

Author

Surin VL, Tagiev AF, Solov'ev GIa, Luk'ianenko AV, Plutalov OV, and Berlin IuA

Subjects

Azerbaijan epidemiology, Base Sequence, Codon, Female, Genetic Markers, Globins genetics, Humans, Male, Molecular Sequence Data, Polymerase Chain Reaction, Polymorphism, Genetic, Pregnancy, beta-Thalassemia prevention & control, Genetic Carrier Screening methods, Mutation, Prenatal Diagnosis methods, beta-Thalassemia genetics

Abstract

Prenatal DNA-diagnosis of beta-thalassemia in a family from Azerbaijan revealed two mutations new for this region--G-A transition at codon 15 and G-C transversion at position 5 of the intron 1. Prenatal diagnosis was carried out by direct sequencing of in vitro amplified (PCR) beta-globin gene fragments with a modified Sanger technique using thermostable DNA polymerase. The absence of parents mutations in the fetal DNA allowed us to conclude that the fetus is normal. The diagnosis was proved at hematological testing of the baby borne.

Published

1993

41. [A PCR-system of analyzing polymorphic markers in gamma-A and gamma-G globin genes and gene for human blood coagulation factor IX with an internal control of the completeness of restriction hydrolysis].

Author

Luk'ianenko AV, Surin VL, Voskoboeva EIu, Tagiev AF, Krutov AA, and Solov'ev GIa

Subjects

Base Sequence, Deoxyribonuclease HindIII, Deoxyribonucleases, Type II Site-Specific, Genetic Markers, Humans, Hydrolysis, Molecular Sequence Data, Polymerase Chain Reaction, Restriction Mapping, Factor IX genetics, Globins genetics, Polymorphism, Restriction Fragment Length

Abstract

New systems are proposed for the PCR analysis of HindIII polymorphic sites in the gamma A and gamma G globin genes and of TaqI polymorphic site in the human factor IX gene of blood population. DNA fragments amplified according to the systems described contain constant restriction site of the appropriate endonuclease, in addition to the polymorphic one, which significantly improves the reliability of the RELP analysis. The systems proposed are highly specific and may be used for DNA diagnosis of beta-thalassemia and haemophilia B.

Published

1993

42. [The introduction of the marker gene Neor into hematopoietic stem cells by electroporation].

Author

Drize NI, Gan OI, and Surin VL

Subjects

Animals, Bone Marrow drug effects, Bone Marrow Cells, Cells, Cultured cytology, Cells, Cultured drug effects, Colony-Forming Units Assay, Electroporation instrumentation, Female, Fluorouracil pharmacology, Gene Transfer Techniques, Genetic Markers genetics, Hematopoietic Stem Cells drug effects, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Plasmids genetics, Time Factors, Electroporation methods, Hematopoietic Stem Cells cytology

Abstract

An electroporation method has been used to introduce marker gene Neor into mouse stem hemopoietic cells which are capable of long-term hemopoiesis maintenance in marrow long-term cultures. Integration of the gene was tested by polymerase chain reaction. The effect of the procedure averaged 50-80% of marked CFUc. Electroporation did little damage to hemopoietic cell precursors. Gene transfer can be made most effectively using bone marrow from mice injected 5-fluorouracil 4 days prior to the experiment.

Published

1993

43. The spectrum of beta-thalassemia mutations in Azerbaijan.

Author

Tagiev AF, Surin VL, Gol'tsov AA, Lukianenko AV, Solovyev GYa, Gulieva EA, Plutalov OV, Kaboev OK, Mamedova TA, and Dadasheva TS

Subjects

Alleles, Azerbaijan, Base Sequence, Child, DNA genetics, DNA Mutational Analysis, Frameshift Mutation, Globins genetics, Humans, Molecular Sequence Data, Point Mutation, Sequence Deletion, Mutation, beta-Thalassemia genetics

Published

1993

44. [A case of prenatal diagnosis of beta-thalassemia by polymerase chain reaction].

Author

Kolesnikova TN, Moliaka IuK, Surin VL, Luk'ianenko AV, Asanov AIu, Tagiev AF, and Solov'ev GIa

Subjects

Base Sequence, DNA, Single-Stranded, Female, Fetal Diseases diagnosis, Globins genetics, Heterozygote, Humans, Molecular Sequence Data, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, Pregnancy, Sequence Deletion, Prenatal Diagnosis, beta-Thalassemia diagnosis

Abstract

The prenatal diagnosis of beta-thalassemia in the Udin family, where the parents were the carriers of 2 bp deletion in the codon 8 (-AA) was undertaken using PCR. Five polymorphic restriction endonuclease sites in the beta-globin gene region were tested. They are: 2 HindIII sites in the gamma G and gamma A genes, 2 HincII sites located in the pseudogene and in its 3'-flanking region, and the AvaIII site in the second exon of the beta-globin gene. The heteroduplex analysis was also performed. Two HindIII polymorphic sites were informative and the HincII site in the pseudogene and the AvaII site in the beta-globin gene were partially informative. According to the results of the RFLP analysis, the embryo was heterozygous. The similar result was obtained by heteroduplex analysis.

Published

1992

45. [Molecular nature of beta-thalassemia in Tajikistan: a four base pair deletion in codons 41-42 of the beta-globin gene].

Author

Kolesnikova TN, Surin VL, Moliaka IuK, Luk'ianenko AV, Tagiev AF, Asanov AIu, Bobokhodzhaev ZM, and Solov'ev GIa

Subjects

Base Sequence, Electrophoresis, Polyacrylamide Gel, Humans, Molecular Sequence Data, Mutation genetics, Polymerase Chain Reaction, Tajikistan ethnology, beta-Thalassemia ethnology, Base Composition genetics, Codon genetics, Gene Deletion, Globins genetics, beta-Thalassemia genetics

Abstract

Thirty tajiks, whose relatives had beta-thalassemia traits (revealed in previous investigations by determination of the HbA-2 and HbF levels) were selected to screen beta-thalassemia mutations. DNA samples from each individual were subjected to the PCR (polymerase chain reaction) to amplify the 635 bp beta-globin gene fragment. One additional band was detected in three samples after the amplified fragment underwent electrophoresis in 2% agarose gel and the EtBr was stained, and two additional ones were revealed by 6% PAAGE and staining of the EtBr. All additional bands migrated more slowly than appropriate 635 bp fragment. It is supposed that additional bands are heteroduplexes formed from the wild type chains and mutated chains carrying a deletion or insertion. The 4 bp deletion of the 41-42 (-tctt) was detected after the direct sequencing of the amplified fragments. This mutation is common among Chinese but it was not revealed in the Middle Asia populations. The mutation can be easily screened using the PCR and electrophoresis in 2% agarose gel or PAAG of the amplified beta-globin gene fragments.

Published

1992

46. Gene therapy model for stromal precursor cells of hematopoietic microenvironment.

Author

Drize NJ, Surin VL, Gan OI, Deryugina EI, and Chertkov JL

Subjects

Animals, Cell Line, Transformed, Cells, Cultured, Female, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Subrenal Capsule Assay, Bone Marrow Cells, Colony-Forming Units Assay methods, Hematopoiesis, Transduction, Genetic physiology, Transfection genetics

Abstract

Marker bacterial Neor gene was transduced by retroviral gene transfer into stromal precursor cells making up the hematopoietic microenvironment in murine long-term bone marrow cultures (LTBMC). Cultures were infected six times during the first 3 weeks of cultivation. At 4 weeks, the adherent cell layers (ACLs) were implanted under the renal capsule of syngeneic unirradiated and irradiated mice. Cells from newly formed ectopic foci were explanted into secondary LTBMC. ACLs containing the marker gene were detected by polymerase chain reaction. About 74% of stromal cells in ACLs contained Neor gene. The possibility of stable gene transduction into stromal precursor cells competent to transfer the hematopoietic microenvironment was established.

Published

1992

47. [Transduction of a marker gene (Neor) into precursor cells of the hematopoietic microenvironment].

Author

Drize NI, Surin VL, Gan OI, Deriugina EI, and Chertkov IL

Subjects

Animals, Cells, Cultured, DNA analysis, DNA genetics, Female, Genetic Markers genetics, Genetic Vectors genetics, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Plasmids genetics, Polymerase Chain Reaction, Retroviridae genetics, Genes, Bacterial genetics, Hematopoietic Stem Cells ultrastructure, Transduction, Genetic genetics

Abstract

The attempt of retroviral transfer of the bacterial Neor gene into stromal precursor cells able to transfer haemopoietic microenvironment and to long-term support of haemopoiesis in vitro and in vivo was made. The existence of marker gene in stromal cells was established by the method of polymerase chain reaction. The transduced stromal precursor cells create normal haemopoietic microenvironment. The data obtained would be important for the further investigation of proliferation and differentiation of stromal precursor cells.

Published

1991

48. [Oncogene-directed mutagenesis in vivo. Polyalkylating derivatives of short single-stranded polynucleotides, complementary E1-adeno-oncogene, in the normalization of adenovirus-transformed rodent cell lines].

Author

Pantin VI, Solov'ev GIa, Sats NV, Surin VL, Borovkova TV, Krutov AA, Zhukova EL, and Grineva NI

Subjects

Adenoviruses, Simian, Alkylating Agents, Animals, Cell Line, Transformed, Cell Transformation, Viral, DNA, Single-Stranded metabolism, Nucleic Acid Hybridization, Phenotype, Polymerase Chain Reaction, Rodentia, DNA, Single-Stranded genetics, Mutagenesis, Site-Directed, Oncogenes

Abstract

Polyalkylating derivatives of single-stranded polynucleotides (30-200-mers) complementary to the long E1 oncogene sequences of simian adenovirus SA7 cause inherited normalization of SH2 and G11 cells transformed with adenovirus SA7; certain deletions in the integrated proviral E1A oncogene were observed in several cases during this process. The transformed cells are indifferent to reagents noncomplementary to the E1 region. Thus polyalkylating derivatives of single-stranded 30-200-mers act as addressed mutagenes which react in a specific way with the integrated complementary DNA sequences of E1 oncogene in transformed rodent cells and realize oncogene-directed mutagenesis in vivo. During this treatment temporary normalized cells reverting to the initial transformed phenotype are also produced.

Published

1991

49. [Penetration of oligo/polynucleotides and their polyalkylating derivatives into rat cells transformed by simian adenovirus DNA].

Author

Pantin VI, Sats NV, Surin VL, Egorov LV, Solov'ev GIa, Borovkova TV, and Grineva NI

Subjects

Alkylation, Animals, Biological Transport, Cell Line, Transformed, Cell Transformation, Viral, Endocytosis, Mutagens pharmacokinetics, Rats, Adenoviruses, Simian, DNA, Viral metabolism, Oligonucleotides metabolism

Abstract

The transport regularity of the [32P]-oligo/polynucleotides and their polyalkylating derivatives into SH2 rat cells transformed with SA7 adenovirus DNA was investigated. Derivatives penetrate the SH2 cells and their distribution in the subcellular fractions are proportional to the concentration of reagent in the medium. The transport efficiency of the derivatives is inhibited sharply with cell concentration increase and practically does not depend on the action of cell metabolism inhibitors. The data obtained assumes the mechanism of the derivatives transport to be liquid endocytosis. Being distributed in the cell components the polyalkylating derivatives were accumulated by the cell nuclei up to 10(5)-10(7) molecules per nucleus. Transport efficiency is much greater in the anchored cells than in the suspended ones. Though essential dephosphorylation of the utilized substances is observed in the SH2 cells, part of them maintain native chain length and the 5'-phosphate group after 1 h incubation in nucleic acids obtained from the cell nuclei.

Published

1991

50. [Use of molecular and genetic approaches in prenatal diagnosis and prevention of hemophilia A and Duchenne muscular dystrophy].

Author

Baranov VS, Aseev MV, Gorbunova VN, Ivashchenko TE, Mikhaĭlov AV, Gornostaeva NI, and Surin VL

Subjects

Chorionic Villi Sampling methods, DNA analysis, DNA genetics, DNA Probes, Female, Fetal Diseases genetics, Fetal Diseases prevention & control, Genetic Carrier Screening methods, Hemophilia A genetics, Hemophilia A prevention & control, Humans, Muscular Dystrophies genetics, Muscular Dystrophies prevention & control, Pregnancy, USSR, Fetal Diseases diagnosis, Hemophilia A diagnosis, Muscular Dystrophies diagnosis, Prenatal Diagnosis methods

Abstract

Allele polymorphism has been evaluated using blot hybridization and a polymerase cascade of DNA synthesis in 40 families at high risk of hemophilia A (a total of 147 subjects) and in 15 families with Duchenne's myodystrophy, Heterozygous carriage of hemophilia A was identified or confirmed in 18 and ruled out in 4 close female relatives of probands. Prenatal tests for fetal hemophilia A were performed in 5 women from families with hemophilia A (in the 1st trimester in 2 and in the 2nd trimester in 3). Four diagnoses of hemophilia A were confirmed and 1 was ruled out. The DNA methods proved revealing in 34 of 40 families with hemophilia A and in 11 of 15 families with Duchenne's myodystrophy. Three of 9 probands were found to have a deletion of the proximal gene for Duchenne's myodystrophy in the DNA probe area of XY 1.1. Prospects of screening for heterozygous carriage and prenatal identification of hemophilia A and Duchenne's myodystrophy are discussed.

Published

1990