Evaluation of oocyte competency in bovine and canine species via non-invasive assessment of oocyte quality

Willingham-Rocky, Lauri A.

2008 December 1900

Traditional methods of oocyte selection for in vitro studies have proven inefficient with respect to achieving a level of predictability for competency. In this study, a novel method of oocyte selection was implemented that identified a relationship between oocyte morphological parameters (as defined by a ratio of a shape factor (SF) to average fluorescence intensity (AFI) and AFI, followed by in vitro fertilization (IVF) and in vitro culture (IVC) using the Well of Well (WOW) method to evaluate oocyte competency. Specifically, we used non-cytotoxic fluorescent molecular probes and multiphoton microscopy to non-invasively characterize spatial localization and functional activity of mitochondria, mitochondrial membrane potential (Δψm), and intracellular calcium activity ([Ca2+]i) using rhodamine 123, JC-1 and Fluo-4, AM, respectively in bovine and canine in vitro matured (IVM) oocytes. Comparison of morphological grading with fluorescence intensity yielded similar trends between all grades of oocytes for both species with no visually obvious, distinct characteristic staining that would permit classification of each oocyte as a specific morphological grade. Our studies confirmed that oocyte mitochondria were homogeneously distributed but primarily localized to the peri- and sub-cortical regions of the oocyte at MII stage for both species. Further, heterogeneously polarized mitochondria were localized to the peri- and sub- cortical regions of the oocyte for both species. In bovine oocytes labeled with Fluo-4, AM, levels of [Ca2+]i were either unremarkable, or very low and limited to the peri-cortical areas, just beneath the oolema. For canine MII stage oocytes, levels of [Ca2+]i were within the same range of AFI as bovine. Ranges of fluorescence intensity compatible for optimal embryo development for bovine and optimal fertilization for canine oocytes were 30-300 and 20-35, and 20-30 and 20-25.5 for rhodamine 123 and Fluo-4, AM, respectively. The optimal range for bovine oocytes imaged with JC-1 was 1.25-2.25 and <6 for canine.

oocyte grading

oocyte competence

mitochondria

in vitro fertilization

calcium

oocyte

Organic chlorine in soilwater : Influence of Clear-cuttning and Nitrogen

Fredriksson, Maria

January 2007

<p>Chlorine is one of most common element on earth and it is essential in every living organism, but can also cause problems in the environment. Chlorine can exist both as inorganic (Clin) and organically bound (Clorg). Earlier was the common opinion that Clorg only occurs from anthropogenic sources, but the last years, research has shown that chlorine is a part of the biogeochemical cycle and Clorg also can have natural sources. Many chlorinated substances are poisonous, so the fact that they have a natural source created attention. Fertilizations with nitrogen in forest areas have shown unexpected consequences, such as an increase leakage of nitrogen to ground and surface water. Clear-cutting is a disturbance on the ecosystem and the environment is sensitive for disturbances. Because of the fact that both chlorine and fertilization can be environmental problems and that clear-cutting is a big disturbance in the nature, this study will investigate if there are changes of organic chlorine (Clorg) in soil water after clear-cutting and if fertilization with nitrogen has any influence on the concentration of Clorg. This study was made in a forest area in Värmland, Sweden (Hagfors). Chemical analyses were made in the laboratory though measuring AOX (absorbable organic halogens). The result of this study showed that clear-cutting probably has some effect on the Clorg concentration and that nitrogen doesn’t have any influence.</p>

Organic chlorine

Clorg

clear-cutting

fertilization

AOX

Environmental chemistry

Miljökemi

Economic and environmental implications of a phosphorus standard : 160-sow representative farm in Montgomery County, Missouri /

Lansford, Vernon D.,

January 2001

Thesis (Ph. D.)--University of Missouri-Columbia, 2001. / Typescript. Vita. Includes bibliographical references (leaves 152-159). Also available on the Internet.

Economic and environmental implications of a phosphorus standard 160-sow representative farm in Montgomery County, Missouri /

Lansford, Vernon D.,

January 2001

Thesis (Ph. D.)--University of Missouri-Columbia, 2001. / Typescript. Vita. Includes bibliographical references (leaves 152-159). Also available on the Internet.

A physiological Approach to the study of pseudopod extension in the amoeboid sperm of the nematode Caenorhabditis elegans

Fraire Zamora, Juan Jose.

January 2009

Thesis (Ph. D.)--University of California, Riverside, 2009. / Includes abstract. Available via ProQuest Digital Dissertations. Title from first page of PDF file (viewed March 16, 2010). Includes bibliographical references. Also issued in print.

Human endometrial gene expression profiling and receptivity in patients undergoing in vitro fertilization (IVF) treatment

Liu, Yunao.

January 2009

Thesis (Ph. D.)--University of Hong Kong, 2009. / Includes bibliographical references (leaves 161-197). Also available in print.

The ethical implications of the Levitical incest laws for medically assisted procreation

Hendricks, Mark William,

January 1999

Thesis (M.C.S.)--Regent College, 1999. / Includes abstract and vita. Includes bibliographical references (leaves 180-186).

Roles of VAD1.3 in spermatogenesis and fertilization

Gao, Jing, 高晶

January 2012

　　Vad1.3 is an evolutionarily-conserved, testis-specific gene identified from a retinol-treated Vitamin A-deficiency (VAD) rat model. VAD1.3 is expressed throughout spermiogenesis at the acrosome of spermatids and epididymal spermatozoa, suggesting a role in acrosome biogenesis or acrosome reaction. The present study aimed to explore the functional role of VAD1.3 in spermatogenesis and sperm functions by the cellular and gene-knockout approaches. 　　Double immunofluorescent microscopy confirmed the co-localization of VAD1.3 and syntaxin 1 in mouse spermatids and spermatozoa. Deletion analysis of the Vad1.3 gene in transfected mouse spermatocyte GC2-spd and human cervical cancer HeLa cells revealed a polarized peri-nuclear/Golgi expression pattern for the N-terminal GFP-VAD fusion proteins which contain a bipartite nucleus localization (BNL) motif, but a nuclear expression pattern for the C-terminal GFP-VAD. The N-terminal sequences of VAD1.3 mediated its interaction with syntaxin 1, as demonstrated by both co-localization and co-immunoprecipitation studies. The full-length GFP-VAD co-localized with the Golgi markers and was redistributed into the endoplasmic reticulum after brefeldin A treatment, suggesting that VAD1.3 was recruited through the ER-Golgi-acrosome pathway. 　　Vad1.3+/- mice was previously generated by the conventional knockout approach. The heterozygous mice had normal spermatogenesis during postnatal days and adulthood (6-8 weeks). At the age of 8-19 months, 6 out of 17 heterozygous mice but no wild-type exhibited a decrease in the epididymal sperm count and testicular weight (p < 0.05). Histological analyses unveiled disarrangement of the seminiferous epithelium and sloughing of germ cells, predominantly spermatids, which was mediated partially by apoptosis as a higher percentage of TUNEL-positive cells were detected in these heterozygous mice (p < 0.05). This phenotype was associated with a decrease in the mRNA (p < 0.05) and protein levels of VAD1.3 in the testis. 　　Crossing of the Vad1.3+/- mice produced wild-type and heterozygous offspring in a ratio of 1:3, but no Vad1.3-/- mice were found. There was no significant difference between the heterozygous intercrosses and the wild-type intercrosses in the number of oocytes ovulated, the developmental rate of embryos from zygotes to blastocysts, the number of implantation site, resorption site or the offspring could result from defective fertilization between Vad1.3 null gametes rather than developmental lethality. The role of VAD1.3 in fertilization was supported by the inhibitory effects of the anti-VAD1.3 antibody on in vitro fertilization and progesterone-induced acrosome reaction. Immuno-staining revealed that VAD1.3 was present in the acrosome-intact spermatozoa but not in acrosome-reacted spermatozoa, indicating a role of VAD1.3 in ZP-binding or acrosome reaction rather than sperm-egg fusion. In oocytes VAD1.3 was distributed in the cytoplasm near the cortex. litter size. Only a few Vad1.3-/- embryos were found at the zygotic (3.7%) and 2-cell (3%) stages in the heterozygous intercrosses. These findings suggested that the absence of the Vad1.3-/- 　　In sum, VAD1.3 may play important roles in fertilization and spermatogenesis in mice. The BNL motif of VAD1.3 directs its Golgi expression and the N-terminal sequence of the protein mediates its interaction with syntaxin 1. The use of tissue-specific knockout approach may help to answer the functional role of VAD1.3 in future. / published_or_final_version / Obstetrics and Gynaecology / Doctoral / Doctor of Philosophy

Fertilization (Biology)

Spermatogenesis in animals.

Rats as laboratory animals.

The ART of making babies : Turkish IVF patients' experiences of childlessness, infertility and Tüp Bebek

Gürtin-Broadbent, Zeynep Başak

January 2013

No description available.

301

Effect of temperature and relative humidity on pollen germination of Gossypium

Ghebremedhen, Zekarias, 1943-

January 1973

No description available.

Cotton -- Growth.

Plants -- Effect of temperature on.

Plants -- Effect of humidity on.

Fertilization of plants.