Isolation of Sperm and Egg Cells from Pepper

Pepper (Capsicum annuum) pollen is bicellular and contains a vegetative cell and a generative cell, which divides in pollen tubes to form two sperm cells. Sperm cells of pepper were isolated using an in vivo–in vitro method. Hand-pollinated styles were first grown in vivo for several hours, then cut from their base and cultured in vitro until pollen tubes grew from the cut end. When the pollen tubes were transferred to a breaking solution, sperm cells were released from broken tubes. Viable embryo sac cells of pepper were isolated using enzymatic digestion and mechanical dissection. Isolated ovules were digested using cellulase and pectinase for 40 minutes and then transferred to an enzyme-free solution for mechanical dissection. Three cells of the egg apparatus and a central cell were released from a cut at the chalazal end of each ovule by pressing on the micropylar area of the ovule with a microneedle. Optimal isolation conditions included 11% mannitol, 0.04% CaCl2, 1% bovine serum albumin (BSA), 1% cellulase, 1% pectinase, and 0.3% pectolyase. Using this protocol, populations of pepper egg cells, synergids, and central cells were isolated.

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Isolation of living sperm cells and in vitro fusion of Torenia fournieri gametes

International Journal of Horticultural Science ◽

10.31421/ijhs/12/4/684 ◽

2006 ◽

Vol 12 (4) ◽

Author(s):

P. Vági ◽

K. Imre ◽

Z. Kristóf

Keyword(s):

Male Gametophyte ◽

Embryo Sac ◽

Pollen Tubes ◽

Sperm Cells ◽

Torenia Fournieri ◽

Isolation Medium ◽

Vitro Fertilization ◽

Crucial Part

In contrast to most angiosperms, Torenia contains a naked embryo sac and therefore has been considered since many years as an exciting model plant to study the double fertilization process of flowering seed plants. It is thus not surprising that the isolation of protoplasts from the female gametophyte has been reported already 20 years ago by Mol, the isolation of megaspores and megagametophytes has been published by the authors of this manuscript in 1996 and in 1999. The isolation of the male gametophyte and of sperm cells was published by the authors in 2004. The isolation of viable Torenia sperm cells is a crucial part of the elaboration of an in vitro fertilization system. Torenia sperm cells were isolated from in vivo — in vitro cultured pollen tubes. In this system pollen tubes first grow inside a cut style then follow their elongation in a solid isolation medium. The medium contained agarose in order to detain pollen tube contents. Released sperm cells and enzymatically isolated egg cells were collected and handled using glass micropipettes and transmitted to an electrofusion apparatus or polyethylene glycol containing media for fusion probes.

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A in Vivo Assay for Standardizing Heparin Preparations

Thrombosis and Haemostasis ◽

10.1055/s-0038-1646810 ◽

1979 ◽

Vol 41 (03) ◽

pp. 576-582

Author(s):

A R Pomeroy

Keyword(s):

In Vitro Assays ◽

British Pharmacopoeia ◽

In Vitro Method ◽

Standard Preparation ◽

Reliable Estimation ◽

Assay Procedure ◽

Accuracy And Precision ◽

Heparin Preparation

SummaryThe limitations of currently used in vitro assays of heparin have demonstrated the need for an in vivo method suitable for routine use.The in vivo method which is described in this paper uses, for each heparin preparation, four groups of five mice which are injected intravenously with heparin according to a “2 and 2 dose assay” procedure. The method is relatively rapid, requiring 3 to 4 hours to test five heparin preparations against a standard preparation of heparin. Levels of accuracy and precision acceptable for the requirements of the British Pharmacopoeia are obtained by combining the results of 3 to 4 assays of a heparin preparation.The similarity of results obtained the in vivo method and the in vitro method of the British Pharmacopoeia for heparin preparations of lung and mucosal origin validates this in vivo method and, conversely, demonstrates that the in vitro method of the British Pharmacopoeia gives a reliable estimation of the in vivo activity of heparin.

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In vitro assessment of food-derived-glucose bioaccessibility and bioavailability in bicameral cell culture system

Turkish Journal of Biochemistry ◽

10.1515/tjb-2020-0082 ◽

2020 ◽

Vol 45 (5) ◽

pp. 631-637

Author(s):

Cansu Ozel-Tasci ◽

Gozde Pilatin ◽

Ozgur Edeer ◽

Sukru Gulec

Keyword(s):

Cell Culture ◽

Culture System ◽

Metabolic Diseases ◽

Enzymatic Digestion ◽

Cell Culture System ◽

Culture Studies ◽

Experimental Approaches ◽

In Vitro Assessment

AbstractBackgroundFunctional foods can help prevent metabolic diseases, and it is essential to evaluate functional characteristics of foods through in vitro and in vivo experimental approaches.ObjectiveWe aimed to use the bicameral cell culture system combined with the in vitro digestion to evaluate glucose bioavailability.Materials and methodsCake, almond paste, and pudding were modified by adding fiber and replacing sugar with sweeteners and polyols. Digestion process was modeled in test tubes. Rat enterocyte cells (IEC-6) were grown in a bicameral cell culture system to mimic the physiological characteristics of the human intestine. The glucose bioaccessibility and cellular glucose efflux were measured by glucose oxidase assay.Results and discussionThe glucose bioaccessibilities of modified foods were significantly lower (cake: 2.6 fold, almond paste: 9.2 fold, pudding 2.8 fold) than the controls. Cellular glucose effluxes also decreased in the modified cake, almond paste, and pudding by 2.2, 4, and 2 fold respectively compared to their controls.ConclusionOur results suggest that combining in vitro enzymatic digestion with cell culture studies can be a practical way to test in vitro glucose bioaccessibility and bioavailability in functional food development.

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Prunus necrotic ringspot virus Early Invasion and Its Effects on Apricot Pollen Grain Performance

Phytopathology ◽

10.1094/phyto-97-8-0892 ◽

2007 ◽

Vol 97 (8) ◽

pp. 892-899 ◽

Cited By ~ 24

Author(s):

Khalid Amari ◽

Lorenzo Burgos ◽

Vicente Pallas ◽

María Amelia Sanchez-Pina

Keyword(s):

Developmental Stages ◽

Generative Cell ◽

Pollen Grains ◽

Growth Zone ◽

Pollen Tubes ◽

Climatic Conditions ◽

Pollen Grain ◽

Ringspot Virus ◽

Prunus Necrotic Ringspot Virus

The route of infection and the pattern of distribution of Prunus necrotic ringspot virus (PNRSV) in apricot pollen were studied. PNRSV was detected both within and on the surface of infected pollen grains. The virus invaded pollen during its early developmental stages, being detected in pollen mother cells. It was distributed uniformly within the cytoplasm of uni- and bicellular pollen grains and infected the generative cell. In mature pollen grains, characterized by their triangular shape, the virus was located mainly at the apertures, suggesting that PNRSV distribution follows the same pattern as the cellular components required for pollen tube germination and cell wall tube synthesis. PNRSV also was localized inside pollen tubes, especially in the growth zone. In vitro experiments demonstrated that infection with PNRSV decreases the germination percentage of pollen grains by more than half and delays the growth of pollen tubes by ≈24 h. However, although PNRSV infection affected apricot pollen grain performance during germination, the presence of the virus did not completely prevent fertilization, because the infected apricot pollen tubes, once germinated, were able to reach the apricot embryo sacs, which, in the climatic conditions of southeastern Spain, mature later than in other climates. Thus, infected pollen still could play an important role in the vertical transmission of PNRSV in apricot.

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Foliar Application of Boron to Almond Trees Affects Pollen Quality

Journal of the American Society for Horticultural Science ◽

10.21273/jashs.125.2.265 ◽

2000 ◽

Vol 125 (2) ◽

pp. 265-270 ◽

Cited By ~ 29

Author(s):

A.M.S. Nyomora ◽

P.H. Brown ◽

K. Pinney ◽

V.S. Polito

Keyword(s):

Pollen Germination ◽

Foliar Application ◽

Culture Media ◽

Pollen Viability ◽

Prunus Dulcis ◽

Pollen Tubes ◽

Tube Growth ◽

Mature Trees

The effect of boron (B) on in vivo and in vitro development of almond [Prunus dulcis (Mill.) D.A. Webb (syn. P. amygdalus Batsch)] pollen and pollen tubes and the resultant effect on fruit set was studied in mature trees. The cultivars Mono (pistil donor) and Butte (pollinizer) in an orchard with low soil B in Fresno, California were sprayed with B at 0, 0.8, 1.7, or 2.5 kg·ha-1 during Fall 1993. Pollen viability as indicated by the fluorescein diacetate method (FDA) was >85% and was not affected by field-applied B, however, in vivo pollen germination and tube growth were enhanced by foliar-applied B. More effect of applied B on in vivo growth appeared as pollen tubes progressed toward the ovary. For in vitro germination, foliar-applied B reduced bursting of tubes, and addition of B to the culture media significantly increased pollen germination and pollen tube growth.

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Hypno-desensitization therapy of vaginismus: Part I. “in vitro” method. Part II. “in vivo” method

International Journal of Clinical and Experimental Hypnosis ◽

10.1080/00207147308409119 ◽

1973 ◽

Vol 21 (3) ◽

pp. 144-156 ◽

Cited By ~ 29

Author(s):

K. Fuchs ◽

Z. Hoch ◽

E. Paldi ◽

H. Abramovici ◽

J. M. Brandes ◽

...

Keyword(s):

In Vitro Method ◽

Desensitization Therapy

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Temperature effects on morphological integrity and Ca2+ signaling in freshly isolated murine feed artery endothelial cell tubes

AJP Heart and Circulatory Physiology ◽

10.1152/ajpheart.00214.2011 ◽

2011 ◽

Vol 301 (3) ◽

pp. H773-H783 ◽

Cited By ~ 19

Author(s):

Matthew J. Socha ◽

Chady H. Hakim ◽

William F. Jackson ◽

Steven S. Segal

Keyword(s):

Endothelial Cell ◽

Enzymatic Digestion ◽

Receptor Activation ◽

Abdominal Muscle ◽

Fura 2 ◽

Intracellular Ca ◽

Feed Arteries ◽

In Vitro Stability

To study Ca2+ signaling in the endothelium of murine feed arteries, we determined the in vitro stability of endothelial cell (EC) tubes freshly isolated from abdominal muscle feed arteries of male and female C57BL/6 mice (5–9 mo, 25–35 g). We tested the hypothesis that intracellular Ca2+ concentration ([Ca2+]i) responses to muscarinic receptor activation would increase with temperature. Intact EC tubes (length: 1–2 mm, width: 65–80 μm) were isolated using gentle enzymatic digestion with trituration to remove smooth muscle cells. A freshly isolated EC tube was secured in a chamber and superfused at 24 (room temperature), 32, or 37°C. Using fura-2 dye, [Ca2+]i was monitored (ratio of fluorescence at 340- to 380-nm wavelength) at rest and in response to bolus doses of ACh (20 nmol to 200 μmol). The morphological integrity of EC tubes was preserved at 24 and 32°C. Based on the Ca2+ Kd values we determined for fura-2 (174 nM at 24°C and 146 nM at 32°C), resting [Ca2+]i remained stable for 180 min at both 24 and 32°C (27 ± 4 and 34 ± 2 nM, respectively), with peak responses to ACh (20 μmol) increasing from ∼220 nM at 24°C to ∼500 nM at 32°C ( P < 0.05). There was no difference in responses to ACh between EC tubes from male versus female mice. When EC tubes were maintained at 37°C (typical in vivo temperature), resting [Ca2+]i increased by ∼30% within 15 min, and gaps formed between individual ECs as they retracted and extruded dye, precluding further study. We conclude that EC tubes enable Ca2+ signaling to be evaluated in the freshly isolated endothelium of murine feed arteries. While Ca2+ responses are enhanced by approximately twofold at 32 versus 24°C, the instability of EC tubes at 37°C precludes their study at typical body temperature.

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Tracking Decitabine Incorporation into Malignant Myeloid Cell DNA in vitro and in vivo by LC-MS/MS with Enzymatic Digestion

Scientific Reports ◽

10.1038/s41598-019-41070-y ◽

2019 ◽

Vol 9 (1) ◽

Cited By ~ 2

Author(s):

Sujatha Chilakala ◽

Ye Feng ◽

Lan Li ◽

Reda Mahfouz ◽

Ebrahem Quteba ◽

...

Keyword(s):

Myeloid Cell ◽

Enzymatic Digestion

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In Vitro Effect of Erythropoietin on the Spleen of The Polycythemic Mouse

Blood ◽

10.1182/blood.v29.6.852.852 ◽

1967 ◽

Vol 29 (6) ◽

pp. 852-858

Author(s):

YASUSADA MIURA ◽

FUMIMARO TAKAKU ◽

KIKU NAKAO

Keyword(s):

Tissue Culture ◽

Culture Method ◽

Stem Cell Differentiation ◽

Mouse Spleen ◽

In Vitro Method ◽

Heme Synthesis ◽

Tissue Culture Method ◽

Vitro Effect

Abstract 1. An in vitro method to observe radiosensitivity of stem cells was developed in the present study. In vivo and in vitro effect of 60Co irradiation on the erythropoietin-induced stem cell differentiation into erythroblasts was observed, using a tissue culture method of polycythemic mouse spleen. Response to erythropoietin was demonstrated by an appearance of heme synthesis and erythroblasts in spleen fragments. 2. A significant correlation between the rate of appearance of erythroblasts and heme synthesis of the spleen fragments was observed. 3. After irradiation, marked impairment of both heme synthesis and production of erythroblasts was observed, yielding D37 values in the vicinity of 70 r in vivo and 120 r in vitro irradiation, respectively. 4. Marked recovery of erythropoietin-induced heme synthesis in the polycythemic mouse spleen was observed 9 days after 300 r irradiation, with an "overshooting" phenomenon on the 12th day.

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Dephosphorylation of protamine 2 at serine 56 is crucial for murine sperm maturation in vivo

Science Signaling ◽

10.1126/scisignal.aao7232 ◽

2019 ◽

Vol 12 (574) ◽

pp. eaao7232 ◽

Cited By ~ 3

Author(s):

Katsuhiko Itoh ◽

Gen Kondoh ◽

Hitoshi Miyachi ◽

Manabu Sugai ◽

Yoshiyuki Kaneko ◽

...

Keyword(s):

Posttranslational Modification ◽

Sperm Maturation ◽

Sperm Cells ◽

Chromatin Binding ◽

Wild Type ◽

Underlying Mechanisms ◽

Deficient Mice ◽

Protamine 2

The posttranslational modification of histones is crucial in spermatogenesis, as in other tissues; however, during spermiogenesis, histones are replaced with protamines, which are critical for the tight packaging of the DNA in sperm cells. Protamines are also posttranslationally modified by phosphorylation and dephosphorylation, which prompted our investigation of the underlying mechanisms and biological consequences of their regulation. On the basis of a screen that implicated the heat shock protein Hspa4l in spermatogenesis, we generated mice deficient in Hspa4l (Hspa4l-null mice), which showed male infertility and the malformation of sperm heads. These phenotypes are similar to those of Ppp1cc-deficient mice, and we found that the amount of a testis- and sperm-specific isoform of the Ppp1cc phosphatase (Ppp1cc2) in the chromatin-binding fraction was substantially less in Hspa4l-null spermatozoa than that in those of wild-type mice. We further showed that Ppp1cc2 was a substrate of the chaperones Hsc70 and Hsp70 and that Hspa4l enhanced the release of Ppp1cc2 from these complexes, enabling the freed Ppp1cc2 to localize to chromatin. Pull-down and in vitro phosphatase assays suggested the dephosphorylation of protamine 2 at serine 56 (Prm2 Ser56) by Ppp1cc2. To confirm the biological importance of Prm2 Ser56 dephosphorylation, we mutated Ser56 to alanine in Prm2 (Prm2 S56A). Introduction of this mutation to Hspa4l-null mice (Hspa4l−/−; Prm2S56A/S56A) restored the malformation of sperm heads and the infertility of Hspa4l−/− mice. The dephosphorylation signal to eliminate phosphate was crucial, and these results unveiled the mechanism and biological relevance of the dephosphorylation of Prm2 for sperm maturation in vivo.

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