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Nesterboy [21]
2 years ago
14

Explain the process of mitosis in a tissue culture for normal cells.

Biology
2 answers:
kari74 [83]2 years ago
8 0
It is when cell chromosomes are separated into two new nuclei.
stira [4]2 years ago
4 0

Mitosis is a process of cell division that results in the production of two cells with identical genetic heritage.

prophase

Prophase (2n-4c) is the first phase of cell division (and the longest, about 90% of dividing time) in mitosis.

1. The centrosomes, consisting of two centrioles (nine triplets of microtubules), each migrate to a pole of the cell.

The microtubule cytoskeleton forms the mitotic spindle (division spindle) that connects the two centrosomes.

2. The chromatin condenses enchromosome, that is to say, into two sister chromatids produced by the replication of the starting chromatid and which contain identical genetic information.

3. The nuclear membrane disintegrates by phosphorylation of the lamins of the nuclear lamina.

4. Kinetochores are formed at the centromere level.

This third part of prophase is called prometaphase and can be defined as an independent phase by some authors.

metaphase

The metaphase (2n-4c) is the phase where the chromosomes are placed on both sides of the equatorial plane to form the equatorial plate.

During this phase especially, but also already in prophase, the chromatin is especially present in compacted form (heterochromatin), resistant form especially around the centromeres: this makes it possible to increase the resistance of the chromosomes to avoid their rupture during their separation during the anaphase.

On the other hand, some regions are poorly compacted (euchromatin).

These gene promoter regions were active in the cell prior to entry into mitosis.

This process called "bookmarking" (gene or mitotic bookmarking, literally: mark page), is an epigenetic mechanism that allows to transmit to the cells cells the "memory" of the active genes before the entry into mitosis. Let's not forget that transcription stops during mitosis.

anaphase

Anaphase (2n-4c) is the phase where sister chromatids separate and migrate to opposite poles of the cell.

It is the sister chromatids that are separated, but not the chromatid pairs as in meiosis.

telophase

Telophase (2n-1c) is the phase in which the nuclear and cellular envelopes appear, leading to the appearance of two cells with 2n chromosomes and each with a chromatide.

During this period, or sometimes, according to the authors, in a last period, called cytokinesis or cytodiérèse, appears a division in a plane perpendicular to the axis of the mitotic spindle which separates the cell in two. This contractile ring is formed of actin and myosin.

All other organelles reform as nucleoli and chromatids decondensate to reform chromatin.

Regulation of the cell cycle

To ensure, on the one hand, the immutable order of the succession of the four phases of the cycle (regulation of the cycle), and on the other hand, the obtaining of two exactly identical daughter cells (DNA monitoring), the cell has highly sophisticated control systems. In the first case, (cycle regulation), it is mainly cyclin-dependent kinases, the Cdk, which intervene. In the second case, other molecules intervene in different mechanisms of cycle monitoring to inhibit the Cdk of the cycle regulation and stop the cycle, if the previous step is not completed, or if a "repair" is necessary .

* The regulation of the succession of the four phases of the cell cycle

The different phases of the cycle take place according to the immutable order mentioned above and it is to ensure the maintenance of this sequence that Cdks that regulate the cell cycle intervene. There are several; they intervene throughout the cycle in a specific order: in phase G1 and for the transition G1-S, that is to say for the triggering of the replication of the DNA, in phase S for the continuation of the replication , in the G2 phase and for the G2-M transition, that is to say for the triggering of the mitosis and for the execution of the mitosis. Cdk act either on the proteins that allow the realization of the events of the cycle (their function is then to cause the events of the cycle), or on the protein Rb, (their function then being to allow the progression of the cycle).

The normal succession of the different phases can take place only if the different Cdk intervening during the different phases are present and active at the opportune moments.


* Cycle monitoring mechanisms.

The monitoring mechanisms are in addition to the regulation of the succession of the four phases of the cycle by the Cdk. They allow the monitoring of fundamental aspects such as the state of the DNA molecules before, during and after their replication (DDCP = DNA Damage Checkpoint), the total completion of the replication before the entry into mitosis (RCP = Replication Checkpoint ) and the correct positioning of all the chromosomes on the plate.

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<u>Answer:</u>

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- Proper aseptic technique is crucial to ensuring growth of pure bacterial colonies. What is one experimental way you can test y
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Answer:

1. Aseptic techniques can be tested for their suitability by flaming the loop or by using agar slants.

2. Culturing equipment can be sterilized by three methods and these include wet heat, dry heat and filtration.

3. Inoculating needles are used for transferring bacterial culture to a soft agar medium. Inoculating loops are used to transfer culture into liquid medium or plate.

4. Growth plates or agar plates, Liquid media and Stab-tube media are used for growth of bacterial colonies.

Explanation:

1. A-septic techniques can be tested for their suitability by flaming the loop or by using agar slants. The loop is flamed to an extent that it becomes red-hot and is then cooled before picking up the organisms from the bacterial culture to be transferred. The hot loop is kept into the tube for a few seconds before removing the inoculum so that a bacterial aerosol is not produced.

2. Culturing equipment can be sterilized by three methods and these include wet heat, dry heat and filtration. Wet heat method is the most preferred method for sterilizing culture material using an autoclave. The material is heated using pressurized steam in an autoclave; which is an effective procedure for killing microbes, spores and viruses at 100◦C. However, it is interesting to know that pressurized steam has 7 times more heat than water at 100◦C which allows rapid delivery of heat and good penetration for sterilizing dense materials. High pressured steam hydrolyzes bacterial protein and removes any chances of contamination.  

Dry heat method kill microbes by oxidation of cells thus requires more energy and is conducted at a higher temperature of 121◦C for efficient sterilization.  

Filtration is another method of sterilizing liquids without heating and is performed by passing the solution through a filter with a pore diameter of 0.2 µm. The filter material used for sterilization can be heat-fused glass funnels or cellulose membranes. However, viruses can pass through these filters and filtration is not a preferred sterilization method.  

3. Inoculating needles are used for transferring bacterial culture to a soft agar medium because needles supports appropriate spreading of culture and produces growth along the stab line also.  

Inoculating loops are used to transfer culture into liquid medium or plate because it is free following and adequate spreading of culture is not required.  

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In order to expand bacterial culture for the purpose of isolating DNA plasmid, liquid media is used. These liquid cultures allow easy inoculation of growth parameters such as antibiotics, and control of temperature and air pressure.  

Stab tube media is prepared by filling test tube with soft agar and is specifically designed for growth of bacteria in low oxygen conditions. The stab tube allows immersion of inoculation loop into the agar depth where oxygen is extremely low and bacterial colonies can be produced without any shaking of media.  

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