Embryo culture is a component of ''in vitro'' fertilisation where in resultant embryos are allowed to grow for some time in an artificial medium.

Duration

The duration of embryo culture can be varied, conferring different stages of

embryogenesis An embryo ( ) is the initial stage of development for a multicellular organism. In organisms that reproduce sexually, embryonic development is the part of the life cycle that begins just after fertilization of the female egg cell by the male ...

embryo transfer Embryo transfer refers to a step in the process of assisted reproduction in which embryos are placed into the uterus of a female with the intent to establish a pregnancy. This technique - which is often used in connection with in vitro fertili ...

. The main stages at which embryo transfer is performed are cleavage stage (day 2 to 4 after

co-incubation In vitro fertilisation (IVF) is a process of fertilisation in which an egg is combined with sperm in vitro ("in glass"). The process involves monitoring and stimulating the ovulatory process, then removing an ovum or ova (egg or eggs) from t ...

) or the

blastocyst The blastocyst is a structure formed in the early embryonic development of mammals. It possesses an inner cell mass (ICM) also known as the ''embryoblast'' which subsequently forms the embryo, and an outer layer of trophoblast cells called the ...

stage (day 5 or 6 after

). Embryos which reach the day 3 cell stage can be tested for chromosomal or specific genetic defects prior to possible transfer by

preimplantation genetic diagnosis Preimplantation genetic diagnosis (PGD or PIGD) is the genetic profiling of embryos prior to implantation (as a form of embryo profiling), and sometimes even of oocytes prior to fertilization. PGD is considered in a similar fashion to prenatal ...

(PGD). Embryo culture until the blastocyst stage confers a significant increase in

live birth rate Pregnancy rate is the success rate for getting pregnant. It is the percentage of all attempts that leads to pregnancy, with attempts generally referring to menstrual cycles where insemination or any artificial equivalent is used, which may be simpl ...

per

, and there is no evidence of a difference between the groups in cumulative pregnancy rates. Transfer day 2 instead of day 3 after fertilization has no differences in

Monozygotic twinning Twins are two offspring produced by the same pregnancy.MedicineNet > Definition of Twin Last Editorial Review: 19 June 2000 Twins can be either ''monozygotic'' ('identical'), meaning that they develop from one zygote, which splits and forms two e ...

is not increased after blastocyst transfer compared with

cleavage-stage embryo In embryology, cleavage is the division of cells in the early development of the embryo, following fertilization. The zygotes of many species undergo rapid cell cycles with no significant overall growth, producing a cluster of cells the same siz ...

transfer. There are significantly higher odds of

preterm birth Preterm birth, also known as premature birth, is the Childbirth, birth of a baby at fewer than 37 weeks Gestational age (obstetrics), gestational age, as opposed to full-term delivery at approximately 40 weeks. Extreme preterm is less than 28 ...

(

odds ratio An odds ratio (OR) is a statistic that quantifies the strength of the association between two events, A and B. The odds ratio is defined as the ratio of the odds of event A taking place in the presence of B, and the odds of A in the absence of B ...

1.3) and congenital anomalies (

1.3) among births from embryos cultured until the blastocyst stage compared with cleavage stage.

Characteristics of an optimal embryo culture

The first thing to take into account are the oxygen and carbon dioxide conditions because they must be as similar as the uterus ones as possible. It is for this reason that oxygen has to be at 5% and carbon dioxide at 6% (depending on altitude). On the other hand, temperature must be set at 37 degrees. In addition, the pH levels should be between 7.2 and 7.5. Regarding the incubator, technicians should place one patient per incubator and avoid frequent door opening. Taking into account the number of embryos used in the culture, group embryo culture is recommended, so they can exchange growing factors while time is saved in the lab but embryo fusion is a drawback that has to be taken into account, in fact, after day five embryo fusion is more likely to happen.

Techniques

Culture of embryos can either be performed in an artificial culture medium or in an autologous endometrial coculture (on top of a layer of cells from the woman's own uterine lining). With artificial culture medium, there can either be the same culture medium throughout the period (''monoculture medium''), or a ''sequential system'' can be used, in which the embryo is sequentially placed in different media, with different formulations based on the different concentration and composition of the tubal and uterine fluid in relation to change in the metabolic activity of the embryo during its development. For example, when culturing to the blastocyst stage, one medium may be used for culture to day 3, and a second medium is used for culture thereafter. Single or sequential medium are equally effective for the culture of human embryos to the blastocyst stage. Artificial embryo culture media basically contain glucose, pyruvate, and energy-providing components, but the addition of amino acids, nucleotides, vitamins, and cholesterol improve the performance of embryonic growth and development. Specifically, embryo culture media contain more pyruvate concentration than glucose in the cleavage phase and more glucose concentration than pyruvato in the blastocyst phase. This is because before day 3 the embryo uses the oocyte reserves, however, from day 3 to the blastocyst it starts to express different proteins to continue its development, so it starts to degrade glucose (it needs more glucose in this case). Also substances like antioxidants, antibiotics, macromolecules, hormones and growth factors can be added. Methods to permit dynamic embryo culture with fluid flow and embryo movement are also available. A new method in development uses the uterus as an incubator and the naturally occurring intrauterine fluids as culture medium by encapsulating the embryos in a permeable intrauterine vessel. A review in 2013 meta-analysis of commercially available IVF culture media was unable to identify a specific media that was superior in terms of pregnancy outcome. Usage of low oxygen concentrations of 5% rather than about 20% in the atmosphere has been shown to increase live birth rate to a relative probability of 1.24, without any evidence of increased risk for multiple pregnancies, miscarriages or congenital abnormalities.

Buffering system

Control and regulation of pH are mandatory for in vitro embryo culture. Culture media can be classified according to type of buffer used: CO₂ / bicarbonate - buffered medium: uses the same physiological buffering system surrounding mammalian cells. Require the use of CO₂ incubators at 5-7%; Phosphate-buffered medium: does not require CO₂ environment. Seems to have detrimental effects in embryo development in vitro; HEPES-buffered medium: used as buffered medium for human oocyte collection and embryo handling; MOPS-buffered medium: like HEPES, has the potential advantage that the buffering capacity is less temperature dependent.

Temperature

While it has been hypothesized that incubating at a temperature lower than 37 °C may be a more accurate recreation of the temperature in the female reproductive tract, the evidence is uncertain whether different temperatures for embryo culture have different effects on pregnancy or live birth rates.

Risks

Animal studies have detected

epigenetic In biology, epigenetics is the study of changes in gene expression that happen without changes to the DNA sequence. The Greek prefix ''epi-'' (ἐπι- "over, outside of, around") in ''epigenetics'' implies features that are "on top of" or "in ...

abnormalities in embryos having undergone embryo culture, indicating a need to optimize the procedures.

Embryo culture in non-human species

In addition to human embryo culture, the technique is employed extensively for non-human species, especially when exploring embryo development,

assisted reproductive technology Assisted reproductive technology (ART) includes medical procedures used primarily to address infertility. This subject involves procedures such as in vitro fertilization (IVF), intracytoplasmic sperm injection (ICSI), and cryopreservation of ga ...

, and the generation of genetically modified animals.

Mouse A mouse (: mice) is a small rodent. Characteristically, mice are known to have a pointed snout, small rounded ears, a body-length scaly tail, and a high breeding rate. The best known mouse species is the common house mouse (''Mus musculus'' ...

embryos, in particular, are frequently cultured for these specific research purposes. The two often used cultural media are potassium simplex optimized medium (KSOM) and '' human tubal fluid'' (HTF). Because KSOM uses a bicarbonate buffering mechanism, it is dependent on a CO₂ incubator to maintain the right pH. As with KSOM, HTF is only appropriate for a CO₂ incubator environment but is employed during the

fertilisation Fertilisation or fertilization (see spelling differences), also known as generative fertilisation, syngamy and impregnation, is the fusion of gametes to give rise to a zygote and initiate its development into a new individual organism or of ...

process. Buffered by a

HEPES HEPES (4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid) is a zwitterionic sulfonic acid buffering agent. It is one of the twenty Good's buffers. HEPES is widely used in cell culture, largely because it is better at maintaining physiological pH ...

system, M2 medium facilitates embryo handling in ambient conditions without the need for CO₂ regulation.

References

{{reflist In vitro fertilisation