Transgenes in F-4 pMThGH-transgenic common carp (Cyprinus carpio L.) are highly polymorphic

To gain information on the integration pattern of pMThGH-transgene, 50 transgenes were recovered from F-4 generation of pMThGH transgenic common carp (Cyprinus carpio L,) and 33 recovered genes were analyzed. The restriction maps of these recovered genes were constructed by digestion with five kinds of enzymes. These transgenes can be classified into 4 types according to their restriction maps. Only one type of transgenes maintains its original molecular form, whereas the other three types are very different from the original one and vary each other on both molecular weight and restriction maps. This implies that the sequences of most transgenes have been deleted and/or rearranged during integration and inheritance. The results of PCR amplification and Southern blot hybridization indicate that MThGH in Type I transgene keeps intact but most of its sequence has been deleted in other three types. All these results suggest that transgenes in F-4 generation of transgenic carp are highly polymorphic. Two DNA fragments concerning integration site of transgenes were cloned from recovered transgenes, and found to be homologous to the 5'UTR of beta -actin gene of common carp and mouse mRNA for receptor tyrosine kinase (RTK), respectively.

Microprojectile bombardment of Laminaria japonica gametophytes and rapid propagation of transgenic lines within a bubble-column bioreactor

A human acidic fibroblast growth factor gene, hafgf, was successfully transferred into Laminaria japonica (kelp) gametophytes via microprojectile bombardment using the biolistic PDS-1000/He gene gun. Following phosphinothricin screening, PCR detection and Southern blot analysis, transgenic L. japonica gametophytes were cultivated in an illuminated bubble-column bioreactor to optimize growth conditions. A maximal final dry cell density of 1,695 mg l(-1) was obtained in a batch culture having an initial dry cell density of 129.75 mg l(-1). This was achieved using an aeration rate of 1.08 l air min(-1) l(-1) culture in a medium containing 1.5 mM inorganic nitrate and 0.15 mM phosphate. In addition, the relationship between different nitrogen sources and growth of transgenic gametophytes indicated that both urea and sodium nitrate were effective nitrogen sources for cell growth, while ammonium ions inhibited growth of these gametophytes.

The integrative expression of GUS gene driven by FCP promoter in the seaweed Laminaria japonica (Phaeophyta)

In this study, the background activity of beta-glucuronidase (GUS) was analyzed histochemically and fluorometrically in the negative control of Laminaria japonica (Phaeophyta) thalli, showing low level of activity. GUS gene transformation without selectable gene in L. japonica was performed using four different promoters, i.e., Cauliflower mosaic virus 35S promoter (CaMV35S) from cauliflower mosaic virus, ubiquitin promoter (UBI) from maize, adenine-methyl transfer enzyme gene promoter (AMT) from virus in green alga Chlorella, and fucoxanthin chlorophyll a/c-binding protein gene promoter (FCP) from diatom Phaeodactylum tricornutum. The GUS transient activity was determined fluorometrically after bombarding sliced parthenogenetic sporophytes explants, and it was found that the activity resulting from CaMV35S and FCP promoters (in 114.3 and 80.6 pmol MU min(-1) (mg protein)(-1), respectively) was higher than for the other two promoters. The female gametophytes were bombarded and regenerated parthenogenetic sporophytes. FCP was the only promoter that resulted in detectable GUS chimeric expression activity during histochemical staining and polymerase chain reaction. Results of Southern blot showed that GUS gene was integrated with the L. japonica genome.

Recombination and heterologous expression of allophycocyanin gene in the chloroplast of Chlamydomonas reinhardtii

Heterogeneous expression of multiple genes in the nucleus of transgenic plants requires the introduction of an individual gene and the subsequent backcross to reconstitute multi-subunit proteins or metabolic pathways. In order to accomplish the expression of multiple genes in a single transformation event, we inserted both large and small subunits of allophycocyanin gene (apcA and apcB) into Chlamydomonas reinhardtii chloroplast expression vector, resulting in papc-S. The constructed vector was then introduced into the chloroplast of C. reinhardtii by micro-particle bombardment. Polymerase chain reaction and Southern blot analysis revealed that the two genes had integrated into the chloroplast genome. Western blot and enzyme-linked immunosorbent assay showed that the two genes from the prokaryotic cyanobacteria could be correctly expressed in the chloroplasts of C. reinhardtii. The expressed foreign protein in transformants accounted for about 2%-3% of total soluble proteins. These findings pave the way to the reconstitution of multi-subunit proteins or metabolic pathways in transgenic C. reinhardtii chloroplasts in a single transformation event.

Establishment of a micro-particle bombardment transformation system for Dunaliella saliva

In this study, we chronicle the establishment of a novel transformation system for the unicellular marine green alga, Dunaliella salina. We introduced the CaMV35S promoter-GUS construct into D. saliva with a PDS1000/He micro-particle bombardment system. Forty eight h after transformation, via histochemical staining, we observed the transient expression of GUS in D. salina cells which had been bombarded under rupture-disc pressures of 450 psi and 900 psi. We observed no GUS activity in either the negative or the blank controls. Our findings indicated that the micro-particle bombardment method constituted a feasible approach to the genetic transformation of D. salina. We also conducted tests of the cells' sensitivity to seven antibiotics and one herbicide, and our results suggested that 20 mu g/ ml of Basta could inhibit cell growth completely. The bar gene, which encodes for phosphinothricin acetyltransferase and confers herbicide tolerance, was introduced into the cells via the above established method. The results of PCR and PCR-Southern blot analyses indicated that the gene was successfully integrated into the genome of the transformants.

Identification of a novel DNA methyltransferase 2 from the brine shrimp, Artemia franciscana

DNA methyltransferase 2 (Dnmt2) is a dual-specificity DNA methyltransferase, which contains a weak DNA methyltransferase and novel tRNA methyltransferase activity. However, its biological function is still enigmatic. To elucidate the expression profiles of Dnmt2 in Artemia franciscana, we isolated the gene encoding a Dnmt2 from A. franciscana and named it as AfDnmt2. The cDNA of AfDnmt2 contained a 1140-bp open reading frame that encoded a putative Dnmt2 protein of 379 amino acids exhibiting 32%similar to 39% identities with other known Dnmt2 homologs. This is the first report of a DNA methyltransferase gene in Crustacean. By using semi-quantitative RT-PCR, A)Dnmt2 was found to be expressed through all developmental stages and its expression increased during resumption of diapause cysts development. Southern blot analysis indicated the presence of multiple copies of AfDnmt2 genes in A. franciscana. (C) 2007 Published by Elsevier Inc.

The recombination and expression of the allophycocyanin beta subunit gene in the chloroplast of Chlamydomonas reinhardtii

A Chlamydomonas reinhardtii (C. reinhardtii) chloroplast expression vector, papc-B, containing the apc-B gene that encodes the beta subunit of the light-harvesting antenna protein allophycocyanin (APC) of cyanobacteria, was constructed and transferred to the chloroplast genome of C. reinhardtii by the biolistic method. The transformants were identified by Southern blot, Western blot and ELISA assays after selection on resistant medium. The recombinant APC beta subunit was expressed in the C. reinhardtii chloroplast and accounted for up to 2-3% (w/w) of the total soluble protein (TSP), suggesting a promising prospect of using C. reinhardtii chloroplasts to produce functional plant-derived proteins.

Expression of beta-carotene hydroxylase gene (crtR-B) from the green alga Haematococcus pluvialis in chloroplasts of Chlamydomonas reinhardtii

A carotenoid gene (crtR-B) from the green alga Haematococcus pluvialis, encoding beta-carotene hydroxylase that was able to catalyze the conversion of beta-carotene to zeaxanthin and canthaxanthin to astaxanthin, was cloned into Chlamydomonas reinhardtii chloroplast expression vector p64D to yield plasmid p64DcrtR-B. The vector p64DcrtR-B was transferred to the chloroplast genome of C. reinhardtii using micro-particle bombardment. PCR and Southern blot analyses indicated that crtR-B was integrated into the chloroplast genome of the transformants. RTPCR assays showed that the H. pluvialis crt R-B gene was expressed in C. reinhardtii transformants. The transformants rapidly synthesized carotenoids in larger quantities than the wild-type upon being transferred from moderate to high-intensity white light. This research provides a foundation for further study to elucidate the possible mechanism of photo-protection by xanthophylls and other carotenoids in high light conditions or through exposure to UV radiation.

两种真核微藻类胡萝卜素代谢工程的初步研究

类胡萝卜素在生物体内具有重要的生理功能，其中虾青素的抗氧化活性、提高动物的免疫能力，预防癌症等生理功能更为显著。类胡萝卜素的代谢工程在大肠杆菌、酵母和高等植物中已取得了较大的进展。本文对真核微藻类胡萝卜素代谢工程进行了初步的探索。 1．克隆雨生红球藻β-胡萝卜素羟化酶基因crtR-B，基因枪法转入衣藻叶绿体，经强光处理转化子，HPLC分析表明细胞的叶黄素库（V＋A＋Z）量较野生型增加，表明是外源的β-胡萝卜素羟化酶将β-胡萝卜素生成玉米黄素。 2．克隆雨生红球藻β-胡萝卜素酮化酶基因bkt，基因枪法转入衣藻叶绿体，RT-PCR及RT-PCR Southern blot分析表明外源基因具有转录活性，但未检测到转化子中积累虾青素。 3．根据盐生杜氏藻大量积累β-胡萝卜素的特点，对其遗传转化体系进行了研究。发现20 µg/ml草丁膦Basta，能够完全抑制1.0×106个/ml细胞生长；通过GUS报告基因在细胞内的瞬时表达，确立了轰击压力450 psi、距离6 cm为基因枪法转化盐生杜氏藻的最佳条件；将bar基因转入细胞，得到稳定的转化子，初步建立了盐生杜氏藻稳定遗传转化体系。克隆了盐生杜氏藻八氢番茄红素合成酶基因psy的cDNA序列、基因组序列及psy基因上游459 bp片段。 本文首次开展了衣藻类胡萝卜素代谢工程研究，发现在强光处理下，衣藻crtR-B转化子外源的羟化酶作用使叶黄素库量增加，实现了对衣藻类胡萝卜素代谢途径的修饰。确立了bar基因为选择标记、Basta为筛选试剂的基因枪转化盐生杜氏藻的遗传转化体系，并克隆了其内源的psy基因5’上游序列，为通过基因工程手段在盐生杜氏藻细胞内积累虾青素奠定了基础。

Manipulación de la senescencia de alfalfa (Medicago sativa L.) por ingeniería genética

En plantas forrajeras como la alfalfa, la senescencia foliar produce tanto una pérdida de la biomasa de forraje como una reducción de la calidad del mismo. Una estrategia molecular para retrasar la senescencia mediante la ingeniería genética se basa en la expresión de la secuencia codificante de la isopentenil transferasa (ipt), enzima clave en la biosíntesis de citoquininas. Para lograrlo resulta crítico la utilización de promotores con expresión no constitutiva que permitan la producción sitio-específica y autorregulada de citoquininas. La manipulación de la senescencia constituye un objetivo particularmente atractivo en especies forrajeras. Se transformaron clones de alfalfa con las construcción AtMYB32-ipt, se logró la regeneración de 3 plantas transgénicas, las cuales fueron confirmadas por PCR al amplificar el transgen ipt. La expresión del transgen se confirmó por RT-PCR y a través de la técnica de Southern blot se observó un patrón de inserción múltiple. También se estableció el patrón de expresión de la construcción AtMYB32-gus, la cual se limitó a los tejidos vasculares, con cierta variabilidad de expresión en la parte aérea las plantas. Los fenotipos observados en las plantas AtMYB32-ipt fueron desde plantas normales a plantas que perdieron la dominancia apical con raíces necrosadas en su mayoría. Se evaluó la senescencia foliar a través de bioensayos de hojas de plantas que incorporaron el transgen ipt y plantas que no lo incorporaron, se observó una senescencia foliar retrasada en plantas transgénicas, se cuantificó dicho retraso a través de los contenidos de clorofila a y b, proteínas foliares totales y cambios en el perfil de las proteínas foliares en geles SDS-PAGE (subunidad mayor de Rubisco). Se observó a los 35 días un mayor contenido de clorofila a y b, proteínas foliares y una mayor intensidad de las bandas de la subunidad mayor de Rubisco en las plantas que incorporaron el transgen ipt

The diversity of extradiol dioxygenase (edo) genes in cresol degrading rhodococci from a creosote-contaminated site that express a wide range of degradative abilities.

Analysis of the bacterial population of soil surface samples from a creosote-contaminated site showed that up to 50% of the culturable micro-organisms detected were able to utilise a mixture of cresols. From fifty different microbial isolates fourteen that could utilise more than one cresol isomer were selected and identified by 16S rRNA analysis. Eight isolates were Rhodococcus strains and six were Pseudomonas strains. In general, the Rhodococcus strains exhibited a broader growth substrate range than the Pseudomonas strains. The distribution of various extradiol dioxygenase (edo) genes, previously associated with aromatic compound degradation in rhodococci, was determined for the Rhodococcus strains by PCR detection and Southern-blot hybridization. One strain, Rhodococcus sp. I1 exhibited the broadest growth substrate range and possessed five different edo genes. Gene disruption experiments indicated that two genes (edoC and edoD) were associated with isopropylbenzene and naphthalene catabolism respectively. The other Rhodococcus strains also possessed some of the edo genes and one (edoB) was present in all of the Rhodococcus strains analysed. None of the rhodococcal edo genes analysed were present in the Pseudomonas strains isolated from the site. It was concluded that individual strains of Rhodococcus possess a wide degradative ability and may be very important in the degradation of complex mixtures of substrates found in creosote.

Identification of a general secretory pathway in a human isolate of Burkholderia vietnamiensis (formerly B. cepacia complex genomovar V) that is required for the secretion of hemolysin and phospholipase C activities

Members of the Burkholderia cepacia complex can secrete proteases, lipases, and hemolysins. We report in this study the identification of a general secretory pathway present in a B. vietnamiensis (formerly genomovar V) clinical isolate, which is required for the efficient secretion of phospholipase C and hemolysin activities. Southern blot hybridization experiments revealed that this general secretion pathway is highly conserved among the different genomovars of the B. cepacia complex and is homologous to a similar system described in B. pseudomallei. We also show that this pathway appears not to be necessary for intracellular survival of B. vietnamiensis within Acanthamoeba polyphaga.

Molecular cloning and expression in Escherichia coli K-12 of chromosomal genes determining the O7 lipopolysaccharide antigen of a human invasive strain of E. coli O7:K1

We have cloned and studied the expression in Escherichia coli K-12 of chromosomal rfb genes determining the biosynthesis of the O7 lipopolysaccharide (LPS) antigen from E. coli K1 strain VW187. Two E. coli K-12 strains carrying recombinant cosmids gave positive coagglutination reactions with protein A-rich staphylococcal particles bearing an O7-specific rabbit polyclonal antiserum. Silver-stained polyacrylamide gels of total membranes extracted with hot phenol showed O side chain material which had O7 specificity as determined by immunoblotting experiments. However, the amount of O7 LPS expressed in E. coli K-12 was considerably lower than that produced by the wild-type strain VW187. Deletion and transposition experiments identified a region of about 17 kilobase pairs which is essential for the expression of O7 LPS. The existence of homologies between the O7 LPS genes and other E. coli O side chain genes was investigated by Southern blot hybridization experiments. An O7-specific probe fragment of 15 kilobase pairs did not hybridize to genomic DNA digests of E. coli strains belonging to several different O types, demonstrating that the O7 LPS genes are unique.

Insights into the role of almond CBF transcription factors in the environmental control of cold acclimation and dormancy break

Dissertation presented to obtain the Ph.D degree in Biology

Untersuchungen zur Verbreitung von Klasse II-Transposons wie Tn21, Tn501 und Tn3 in terrestrischen Habitaten

Mobile genetische Elementen wie Transposons wurden in unbelasteten Böden nachgewiesen. Hierzu wurden unterschiedliche Ansätze gewählt: Verschiedene, unbelastete Böden wurden mittels PCR auf das Vorhandensein von Markergenen, in diesem Fall Transposasen vom Typ Tn3, Tn21 und Tn501, hin untersucht. Hierzu wurde ein System entwickelt, welches es ermöglichte die Gesamt-DNA aus verschiedensten Böden mit einem System einfach und reproduzierbar zu extrahieren und anschließend mittels PCR zu untersuchen. Die mittlere Nachweisgrenze dieses Systems lag bei 9 x 10 *3 Templates / g Boden. Ein paralleler Ansatz erfolgte, indem aus den gleichen, unbelasteten Böden Bakterien mittels Selektivmedien isoliert wurden. Diese Isolate wurden anschließend auf genetische Marker hin untersucht. Transposons, bzw. Transposasen konnten in den unbelasteten Böden in weitaus geringerer Zahl als aus belasteten Böden bekannt nachgewiesen werden. Jedoch verhielten sich die unterschiedlichen Elemente in der Verteilung wie aus belasteten Böden bekannt. Am häufigsten wurde Tn21 dann Tn501 nachgewiesen. Tn3, nach dem auch gescreent wurde, konnte nicht nachgewiesen werden. Anschließend wurden diese Böden mittels Bodensäulen unter Laborbedingungen auf die Übertragung von potentiell transponierbaren Elementen aus der autochthonen Flora hin untersucht. Mittels dieses Experimentes konnte kein transponierbares Element nachgewiesen werden. Weiterhin wurden vorhandene Boden-Bakterienkollektive auf das Vorhandensein von Transposons mittels Gensondentechnik und PCR auf Transposasen hin gescreent. Auch hier konnten wiederum Signale zu Tn21, Tn501 und in diesem Falle auch Tn3 erhalten werden. Einige dieser Isolate wurden mittels Southern-Blot und Sequenzierung näher charakterisiert. Bei den Sequenzvergleichen einer so erhaltenen 2257 bp langen Sequenz wurde diese als Transposase der Tn21-Familie mit großer Homologie zur Transposase von Tn5060 bestimmt.