The application of cDNA and tissue microarray methods in the study of human carcinomas

Currently, numerous high-throughput technologies are available for the study of human carcinomas. In literature, many variations of these techniques have been described. The common denominator for these methodologies is the high amount of data obtained in a single experiment, in a short time period, and at a fairly low cost. However, these methods have also been described with several problems and limitations. The purpose of this study was to test the applicability of two selected high-throughput methods, cDNA and tissue microarrays (TMA), in cancer research. Two common human malignancies, breast and colorectal cancer, were used as examples. This thesis aims to present some practical considerations that need to be addressed when applying these techniques. cDNA microarrays were applied to screen aberrant gene expression in breast and colon cancers. Immunohistochemistry was used to validate the results and to evaluate the association of selected novel tumour markers with the outcome of the patients. The type of histological material used in immunohistochemistry was evaluated especially considering the applicability of whole tissue sections and different types of TMAs. Special attention was put on the methodological details in the cDNA microarray and TMA experiments. In conclusion, many potential tumour markers were identified in the cDNA microarray analyses. Immunohistochemistry could be applied to validate the observed gene expression changes of selected markers and to associate their expression change with patient outcome. In the current experiments, both TMAs and whole tissue sections could be used for this purpose. This study showed for the first time that securin and p120 catenin protein expression predict breast cancer outcome and the immunopositivity of carbonic anhydrase IX associates with the outcome of rectal cancer. The predictive value of these proteins was statistically evident also in multivariate analyses with up to a 13.1- fold risk for cancer specific death in a specific subgroup of patients.

The Role of Integrins in Enterovirus Infections and in Metastasis of Cancer

Integrins are a family of transmembrane glycoproteins, composed of two different subunits (alpha and beta). Altered expression of integrins in tumor cells contributes to metastasis tendency by influencing on the cells‟ attachment to adjacent cells and their migration. Viral pathogens, including certain enteroviruses, use integrins as receptors. Enteroviruses have also been suggested to be involved in the etiopathogenesis of type 1 diabetes. The study focuses on the role of integrins in the pathogenesis of metastasis to cortical bone and on type 1 diabetes (T1D) and echovirus 1 infection. In the first part of the thesis, the role of different integrins in the initial attachment of MDA-MD-231 breast cancer cells to bovine cortical bone disks was studied. A close correlation between alpha2beta1 and alpha3beta1 integrin receptor expression and the capability of the tumor to attach to bone were observed. In the second part, a possible correlation between susceptibility to enterovirus infections in diabetic children and differences in enterovirus receptor genes, including certain integrins, was investigated. In parallel, virus-specific neutralizing antibodies and diabetic risk alleles were studied. In the diabetic group, an amino acid change was detected in the polio virus receptor and the neutralizing antibody titers against echovirus 30 were lower. However, to obtain statistically sustainable results, a larger number of individuals should be analyzed. Echovirus 1 (EV1) enters cells by attaching to the alpha2I domain of the alpha2beta1 integrin. In the third part EV1 was shown to attach to a chimeric receptor construct of the transferrin receptor and the alpha2I domain and to enter cells through clathrin-mediated endocytosis that is normally not used by the virus. The chimeric receptor was recycled to the plasma membrane, whereas the virus remained in intracellular vesicles. The virus replication cycle was initiated in these cells, suggesting that evolution pressure could possibly cause the virus to evolve to use a different entry mechanism. Moreover, a cDNA microarray analysis of host gene expression during EV1 replication showed that 0.53% of the total genes, including several immediate early genes, were differently expressed.

Transcriptional Profiling of Organ‐Specific Autoimmunity in Human

Our understanding of the pathogenesis of organ‐specific autoinflammation has been restricted by limited access to the target organs. Peripheral blood, however, as a preferred transportation route for immune cells, provides a window to assess the entire immune system throughout the body. Transcriptional profiling with RNA stabilizing blood collection tubes reflects in vivo expression profiles at the time the blood is drawn, allowing detection of the disease activity in different samples or within the same sample over time. The main objective of this Ph.D. study was to apply gene‐expression microarrays in the characterization of peripheral blood transcriptional profiles in patients with autoimmune diseases. To achieve this goal a custom cDNA microarray targeted for gene‐expression profiling of human immune system was designed and produced. Sample collection and preparation was then optimized to allow gene‐expression profiling from whole‐blood samples. To overcome challenges resulting from minute amounts of sample material, RNA amplification was successfully applied to study pregnancy related immunosuppression in patients with multiple sclerosis (MS). Furthermore, similar sample preparation was applied to characterize longitudinal genome‐wide expression profiles in children with type 1 diabetes (T1D) associated autoantibodies and eventually clinical T1D. Blood transcriptome analyses, using both the ImmunoChip cDNA microarray with targeted probe selection and genome‐wide Affymetrix U133 Plus 2.0 oligonucleotide array, enabled monitoring of autoimmune activity. Novel disease related genes and general autoimmune signatures were identified. Notably, down‐regulation of the HLA class Ib molecules in peripheral blood was associated with disease activity in both MS and T1D. Taken together, these studies demonstrate the potential of peripheral blood transcriptional profiling in biomedical research and diagnostics. Imbalances in peripheral blood transcriptional activity may reveal dynamic changes that are relevant for the disease but might be completely missed in conventional cross‐sectional studies.

Characterisation of Human Neutral and Lysosomal alpha-Mannosidases

Neutral alpha-mannosidase and lysosomal MAN2B1 alpha-mannosidase belong to glycoside hydrolase family 38, which contains essential enzymes required for the modification and catabolism of asparagine-linked glycans on proteins. MAN2B1 catalyses lysosomal glycan degradation, while neutral α-mannosidase is most likely involved in the catabolism of cytosolic free oligosaccharides. These mannose containing saccharides are generated during glycosylation or released from misfolded glycoproteins, which are detected by quality control in the endoplasmic reticulum. To characterise the biological function of human neutral α-mannosidase, I cloned the alpha-mannosidase cDNA and recombinantly expressed the enzyme. The purified enzyme trimmed the putative natural substrate Man9GlcNAc to Man5GlcNAc, whereas the reducing end GlcNAc2 limited trimming to Man8GlcNAc2. Neutral α-mannosidase showed highest enzyme activity at neutral pH and was activated by the cations Fe₂+, Co2+ and Mn₂+, Cu2+ in turn had a strong inhibitory effect on alpha-mannosidase activity. Analysis of its intracellular localisation revealed that neutral alpha-mannosidase is cytosolic and colocalises with proteasomes. Further work showed that the overexpression of neutral alpha-mannosidase affected the cytosolic free oligosaccharide content and led to enhanced endoplasmic reticulum associated degradation and underglycosylation of secreted proteins. The second part of the study focused on MAN2B1 and the inherited lysosomal storage disorder α-mannosidosis. In this disorder, deficient MAN2B1 activity is associated with mutations in the MAN2B1 gene. The thesis reports the molecular consequences of 35 alpha-mannosidosis associated mutations, including 29 novel missense mutations. According to experimental analyses, the mutations fall into four groups: Mutations, which prevent transport to lysosomes are accompanied with a lack of proteolytic processing of the enzyme (groups 1 and 3). Although the rest of the mutations (groups 2 and 4) allow transport to lysosomes, the mutated proteins are less efficiently processed to their mature form than is wild type MAN2B1. Analysis of the effect of the mutations on the model structure of human lysosomal alpha-mannosidase provides insights on their structural consequences. Mutations, which affect amino acids important for folding (prolines, glycines, cysteines) or domain interface interactions (arginines), arrest the enzyme in the endoplasmic reticulum. Surface mutations and changes, which do not drastically alter residue volume, are tolerated better. Descriptions of the mutations and clinical data are compiled in an α-mannosidosis database, which will be available for the scientific community. This thesis provides a detailed insight into two ubiquitous human alpha-mannosidases. It demonstrates that neutral alpha-mannosidase is involved in the degradation of cytosolic oligosaccharides and suggests that the regulation of this α-mannosidase is important for maintaining the cellular homeostasis of N-glycosylation and glycan degradation. The study on alpha-mannosidosis associated mutations identifies multiple mechanisms for how these mutations are detrimental for MAN2B1 activity. The α-mannosidosis database will benefit both clinicians and scientific research on lysosomal alpha‑mannosidosis.

Pikornavirusten käyttö geenivektoreina ja syöpäterapiassa sekä Coxsackievirus A7 -isolaattien sekvenssianalyysi

Kirjallisessa osassa tarkasteltiin pikornavirusten käyttöä geenivektoreina ja syöpäterapiassa. Pikornavirukset ovat positiivissäikeisiä RNA-viruksia, ja niiden genomi koostuu rakenteellisista kuoriproteiineista VP1-VP4 sekä ei-rakenteellisista proteiineista 2A-2C ja 3A-3D. Geenivektoritutkimukset ovat keskittyneet erilaisten inserttien kloonaamiseen virusten VP1-VP4-alueelle ja genomin 5'-päähän sekä näiden muutosten vaikutusten seuraamiseen virusten elinkierrossa solu- ja hiirimalleissa. Geenivektoreina on parhaiten toimineet coxsackievirukset B3, B4 ja A9 sekä mengo- ja poliovirus. Niitä on käytetty hiirissä mm. neuronien motorisen BDNF-reseptorin ilmentämiseen sekä hiiren interleukiini-10:n tuottamiseen selkäydinkanavan vaurioiden korjaamiseksi. Syöpäterapiatutkimuksissa on saatu lupaavia tuloksia coxsackieviruksilla A21, A13, A15 ja A18 sekä echo-, Seneca Valley 001- ja EMCV-viruksilla. Viruksilla on saatu mm. rintasyövän pääkasvain ja metastasoituneet etäpesäkkeet häviämään sekä eturauhassyövän kasvaimia pienenemään. Seneca Valley 001 -virus on osoittautunut tehokkaaksi syöpiä vastaan, joilla on neuroendokriinisiä ominaisuuksia. Viruksen käyttämistä faasi 2:n kliinisiin kokeisiin ollaan parhaillaan suunnittelemassa pienisoluisen keuhkosyövän ja lasten neuroendokriinisen syövän kohdalla. Kokeellisessa osassa optimoitiin RT-PCR-menetelmä coxsackievirus A7:n (CV-A7) genomin tuottamiseksi PCR-reaktiolla (FL-PCR). FL-PCR:n optimointi tehtiin vektoreilla, joihin oli kloonattu CV-A7-USSR- (USSR-pcDNA3) ja CV-A7-Parkerisolaattien (Parker-TA) genomit. Menetelmää käytettiin myöhemmin muiden CV-A7- virusisolaattien (275/58, ET1080 ja SVK) tutkimiseen. Näistä isolaateista eristettiin virus-RNA, joka käännettiin cDNA:ksi RT-entsyymillä. PCR:ssä käytetyt, CV-A7- spesifiset koettimet oli suunniteltu aiemmin sekvensoidun CV-A7-sekvenssin (GenBank AY421765) pohjalta. Infektiivisen kloonin tuottamiseksi USSR-pcDNA3- ja Parker-TA-vektoreista tuotettiin PCR:n avulla (T7-PCR) virusgenomin sisältävä DNAjakso, jonka 5'-päähän muodostui alukkeiden avulla T7RNA-polymeraasipromoottori ja 3'-päähän polyA-häntä. Työssä myös sekvensoitiin ja analysoitiin CV-A7-virusisolaatit Parker, USSR, 275/58, ET1080 ja SVK sekä kloonattiin täyspitkiä virusgenomeja cDNA-muodossa mutaatiokokeita varten. FL-PCR:n optimointi onnistui, ja neljä viidestä CV-A7-isolaatista sekvensoitiin. Virusgenomien pituus vaihteli 7403–7405 nt:n välillä. CV-A7-ET1080, -Parker ja - USSR osoittautuivat yli 99 % ja CV-A7-275/58 82,6 % nt samankaltaisiksi koko genomin pituudelta AY421765:en suhteen. Yksittäisten geenien ja proteiinien osalta CV-A7-275/58 oli 75,8–90,4 % nt ja 93,7–98,8 % aa samankaltainen muiden suhteen. Simplot-analyysissä 3B-geenialue oli heterogeenisin. CV-A7-SVK-isolaatti osoittautui echovirus kolmeksi. Infektiivistä kloonia ei saatu tuotettua T7-PCR-tuotteista.